Your search keyword '"Dura Mater cytology"' showing total 155 results

1. Protocol to characterize mouse dural mast cells by flow cytometry and immunofluorescence.

Author

Lin CJ, Jaafar N, and Tanzi RE

Subjects

Animals, Mice, Dura Mater cytology, Microscopy, Confocal methods, Mast Cells cytology, Flow Cytometry methods, Fluorescent Antibody Technique methods

Abstract

Mast cells, which constitute tissue-resident immune cells, are distributed in the dural meninges. Here, we provide procedural guidelines for investigating mouse dural mast cells using two techniques. First, we outline the procedures for dural tissue dissection, single-cell isolation, and subsequent surface staining for mast cell identification via flow cytometry. We then describe the techniques employed for whole dura tissue staining to visualize mast cells using confocal and slide scanning microscopy, followed by analysis using Nikon's NIS-Elements Advanced Research software. For complete details on the use and execution of this protocol, please refer to Lin et al. 1 ., Competing Interests: Declaration of interests R.E.T. is an inventor on patents involving the use of the mast cell stabilizer, cromolyn and its analogs, for treatment of COVID (US20230149345A1), cytokine release syndrome (US20220218652A1), and inflammation in neurodegenerative disease (US-11679095-B2 and US-20220079914-A1). R.E.T. also holds equity in AZTherapies, which is developing mast cell stabilizers., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2024

2. The Influence of Extracellular Vesicles Secreted by Dural Cells on Osteoblasts.

Author

Zhao F, Zhu J, Dong X, Guo X, Lai C, Zhao J, Zong X, Song G, and Jin X

Subjects

Animals, Apoptosis, Skull cytology, Skull metabolism, Mice, Male, Cells, Cultured, Extracellular Vesicles metabolism, Osteoblasts metabolism, Osteoblasts cytology, Osteogenesis, Dura Mater metabolism, Dura Mater cytology, Cell Differentiation, Cell Proliferation, Cell Movement

Abstract

To explore the influence of extracellular vesicles secreted by dural cells (Dura-EVs) on osteoblasts. Our methodology involves assessing the effects of these EVs at concentrations of 50ug/ml, 100ug/ml, and 200ug/ml on osteoblasts proliferation, differentiation, migration, osteogenesis, and inhibition of apoptosis. We also treated a cranial defect model with injections of these Dura-EVs and monitored the healing rate of cranial defects. Tissue sections were analyzed using Hematoxylin and Eosin (H & E), Masson's trichrome, and immunofluorescence (IF) staining. Our results suggest that Dura-EVs can enhance osteoblasts proliferation, migration, differentiation, and osteogenesis in a dose-dependent manner in vitro. In vivo, Dura-EVs may promote the repair of skull defects. Dura-EVs have an important influence on osteoblasts, our findings shed light on a novel aspect of the dura mater's contribution to cranial osteogenesis., Competing Interests: Declarations Conflict of interest The authors declare that there have no conflict of interest to disclose. Ethical Approval The privacy rights of animal subjects were observed. Consent to Participate Not applicable. Consent to Publish Not applicable., (© 2023. The Author(s), under exclusive licence to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2024

3. A mesothelium divides the subarachnoid space into functional compartments.

Author

Møllgård K, Beinlich FRM, Kusk P, Miyakoshi LM, Delle C, Plá V, Hauglund NL, Esmail T, Rasmussen MK, Gomolka RS, Mori Y, and Nedergaard M

Subjects

Animals, Humans, Mice, Dura Mater cytology, Dura Mater physiology, Endothelium cytology, Endothelium physiology, Epithelium physiology, Cerebrospinal Fluid physiology, Subarachnoid Space cytology, Subarachnoid Space physiology, Brain anatomy & histology, Brain immunology

Abstract

The central nervous system is lined by meninges, classically known as dura, arachnoid, and pia mater. We show the existence of a fourth meningeal layer that compartmentalizes the subarachnoid space in the mouse and human brain, designated the subarachnoid lymphatic-like membrane (SLYM). SLYM is morpho- and immunophenotypically similar to the mesothelial membrane lining of peripheral organs and body cavities, and it encases blood vessels and harbors immune cells. Functionally, the close apposition of SLYM with the endothelial lining of the meningeal venous sinus permits direct exchange of small solutes between cerebrospinal fluid and venous blood, thus representing the mouse equivalent of the arachnoid granulations. The functional characterization of SLYM provides fundamental insights into brain immune barriers and fluid transport.

Published

2023

4. Proteoglycan 4 is present within the dura mater and produced by mesenchymal progenitor cells.

Author

Mudigonda S, Shah S, Das N, Corpuz JM, Ninkovic N, Al-Jezani N, Underhill TM, Salo PT, Mitha AP, Lyons FG, Cho R, Schmidt TA, Dufour A, and Krawetz RJ

Subjects

Animals, Dura Mater cytology, Humans, Mice, Dura Mater metabolism, Mesenchymal Stem Cells metabolism, Proteoglycans metabolism

Abstract

Mesenchymal progenitor cells (MPCs) have been recently identified in human and murine epidural fat and have been hypothesized to contribute to the maintenance/repair/regeneration of the dura mater. MPCs can secrete proteoglycan 4 (PRG4/lubricin), and this protein can regulate tissue homeostasis through bio-lubrication and immunomodulatory functions. MPC lineage tracing reporter mice (Hic1) and human epidural fat MPCs were used to determine if PRG4 is expressed by these cells in vivo. PRG4 expression co-localized with Hic1 + MPCs in the dura throughout skeletal maturity and was localized adjacent to sites of dural injury. When Hic1 + MPCs were ablated, PRG4 expression was retained in the dura, yet when Prx1 + MPCs were ablated, PRG4 expression was completely lost. A number of cellular processes were impacted in human epidural fat MPCs treated with rhPRG4, and human MPCs contributed to the formation of epidural fat, and dura tissues were xenotransplanted into mouse dural injuries. We have shown that human and mouse MPCs in the epidural/dura microenvironment produce PRG4 and can contribute to dura homeostasis/repair/regeneration. Overall, these results suggest that these MPCs have biological significance within the dural microenvironment and that the role of PRG4 needs to be further elucidated., (© 2022. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published

2022

5. The Effect of Yes-Associated Protein on the Interaction Between the MEK/Extracellular Signal-Regulated Kinase and Hippo Pathways in Osteoblasts Co-Cultured With Fibroblast Growth Factor Receptor 2-Mutated Dura Cells.

Author

Dong X, Zhang M, Li C, Lai C, Song G, and Jin X

Subjects

Animals, Cell Differentiation, Coculture Techniques, Dura Mater cytology, Extracellular Signal-Regulated MAP Kinases metabolism, Hippo Signaling Pathway, Mice, Mice, Inbred C57BL, Mitogen-Activated Protein Kinase Kinases metabolism, Osteoblasts cytology, Receptor, Fibroblast Growth Factor, Type 2 genetics, YAP-Signaling Proteins genetics

Abstract

Background: C342Y (Cys342Tyr) point mutation of FGFR2 (fibroblast growth factor receptor 2) is closely associated with the pathogenesis of Crouzon syndrome. The dura mater plays an important role in mediating the closure of cranial sutures. However, the underlying mechanisms of these pathological processes have been rarely investigated. in this study, the authors analyzed the effects of dura cells with FGFR2 mutations on the biological function of osteoblasts., Methods: Dura cells and cranial osteoblasts from C57BL/6 mice were extracted and cultured. C342Y-FGFR2 mutant constructs were established via lentivirus and applied to infect dura cells. A co-cultured trans-well system with dura cells and osteoblasts was established. Three experimental groups were set up: oste group, Oste + Dura-vector group, and Oste + Dura-C342Y group. The expression levels of key factors in MEK (Mitogen-activated protein kinase kinase, MAPKK)/extracellular signal-regulated kinase (ERK) and Hippo pathway were detected by western blot and RT-qPCR (Real Time Quantitative PCR). Finally, a rescue experiment was carried out with small interference RUA., Results: The proliferation level of osteoblasts in Oste + Dura- C342Y group was significantly up-regulated. Our studies indicated that the activation of MEK/ERK pathway in Oste + Dura-C342Y group could inhibit the Hippo pathway, lead to down-regulation of large tumor suppressor 1 and promote the activation and nuclear localization of yes-associated protein, and the results of rescue experiments showed a reverse expression trend, further confirming the effects of C342Y-FGFR2 mutation in dura cells on osteoblasts and its potential mechanism., Conclusions: This study suggested that the C342Y-FGFR2 mutation in dura cells could promote osteoblastic proliferation, and shown the crosstalk between MEK/ERK and Hippo pathways. As the regulatory machinery center, yes-associated protein might play a bridging role in these pathways, and might influence the pathogenesis of craniosynostosis by activating downstream transcriptional factors., Competing Interests: The authors report no conflicts of interest., (Copyright © 2021 by Mutaz B. Habal, MD.)

Published

2022

6. The developing mouse coronal suture at single-cell resolution.

Author

Farmer DT, Mlcochova H, Zhou Y, Koelling N, Wang G, Ashley N, Bugacov H, Chen HJ, Parvez R, Tseng KC, Merrill AE, Maxson RE Jr, Wilkie AOM, Crump JG, and Twigg SRF

Subjects

Acrocephalosyndactylia embryology, Acrocephalosyndactylia genetics, Acrocephalosyndactylia pathology, Animals, Basic Helix-Loop-Helix Transcription Factors genetics, Basic Helix-Loop-Helix Transcription Factors metabolism, Cranial Sutures cytology, Cranial Sutures embryology, Dura Mater cytology, Dura Mater embryology, Dura Mater metabolism, Mesoderm cytology, Mesoderm embryology, Mesoderm metabolism, Mice, Knockout, Mice, Transgenic, Osteoblasts cytology, Osteoblasts metabolism, RNA-Seq methods, Skull cytology, Skull embryology, Skull metabolism, Twist-Related Protein 1 genetics, Twist-Related Protein 1 metabolism, Mice, Cranial Sutures metabolism, Gene Expression Regulation, Developmental, Osteogenesis genetics, Single-Cell Analysis methods, Transcriptome genetics

Abstract

Sutures separate the flat bones of the skull and enable coordinated growth of the brain and overlying cranium. The coronal suture is most commonly fused in monogenic craniosynostosis, yet the unique aspects of its development remain incompletely understood. To uncover the cellular diversity within the murine embryonic coronal suture, we generated single-cell transcriptomes and performed extensive expression validation. We find distinct pre-osteoblast signatures between the bone fronts and periosteum, a ligament-like population above the suture that persists into adulthood, and a chondrogenic-like population in the dura mater underlying the suture. Lineage tracing reveals an embryonic Six2+ osteoprogenitor population that contributes to the postnatal suture mesenchyme, with these progenitors being preferentially affected in a Twist1+/-; Tcf12+/- mouse model of Saethre-Chotzen Syndrome. This single-cell atlas provides a resource for understanding the development of the coronal suture and the mechanisms for its loss in craniosynostosis., (© 2021. The Author(s).)

Published

2021

7. Skull and vertebral bone marrow are myeloid cell reservoirs for the meninges and CNS parenchyma.

Author

Cugurra A, Mamuladze T, Rustenhoven J, Dykstra T, Beroshvili G, Greenberg ZJ, Baker W, Papadopoulos Z, Drieu A, Blackburn S, Kanamori M, Brioschi S, Herz J, Schuettpelz LG, Colonna M, Smirnov I, and Kipnis J

Subjects

Animals, Bone Marrow physiology, Brain cytology, Brain immunology, Brain physiology, Cell Movement, Central Nervous System cytology, Central Nervous System Diseases pathology, Dura Mater cytology, Dura Mater immunology, Dura Mater physiology, Encephalomyelitis, Autoimmune, Experimental immunology, Encephalomyelitis, Autoimmune, Experimental pathology, Homeostasis, Meninges cytology, Meninges physiology, Mice, Monocytes physiology, Neutrophils physiology, Spinal Cord cytology, Spinal Cord immunology, Spinal Cord physiology, Spinal Cord Injuries immunology, Spinal Cord Injuries pathology, Bone Marrow Cells physiology, Central Nervous System immunology, Central Nervous System Diseases immunology, Meninges immunology, Myeloid Cells physiology, Skull anatomy & histology, Spine anatomy & histology

Abstract

The meninges are a membranous structure enveloping the central nervous system (CNS) that host a rich repertoire of immune cells mediating CNS immune surveillance. Here, we report that the mouse meninges contain a pool of monocytes and neutrophils supplied not from the blood but by adjacent skull and vertebral bone marrow. Under pathological conditions, including spinal cord injury and neuroinflammation, CNS-infiltrating myeloid cells can originate from brain borders and display transcriptional signatures distinct from their blood-derived counterparts. Thus, CNS borders are populated by myeloid cells from adjacent bone marrow niches, strategically placed to supply innate immune cells under homeostatic and pathological conditions. These findings call for a reinterpretation of immune-cell infiltration into the CNS during injury and autoimmunity and may inform future therapeutic approaches that harness meningeal immune cells., (Copyright © 2021 The Authors, some rights reserved; exclusive licensee American Association for the Advancement of Science. No claim to original U.S. Government Works.)

Published

2021

8. Heterogeneity of meningeal B cells reveals a lymphopoietic niche at the CNS borders.

Author

Brioschi S, Wang WL, Peng V, Wang M, Shchukina I, Greenberg ZJ, Bando JK, Jaeger N, Czepielewski RS, Swain A, Mogilenko DA, Beatty WL, Bayguinov P, Fitzpatrick JAJ, Schuettpelz LG, Fronick CC, Smirnov I, Kipnis J, Shapiro VS, Wu GF, Gilfillan S, Cella M, Artyomov MN, Kleinstein SH, and Colonna M

Subjects

Aging, Animals, B-Lymphocyte Subsets immunology, Cell Movement, Central Nervous System physiology, Dura Mater immunology, Fibroblasts physiology, Homeostasis, Immune Privilege, Mice, Plasma Cells physiology, Single-Cell Analysis, B-Lymphocyte Subsets physiology, B-Lymphocytes physiology, Bone Marrow Cells physiology, Central Nervous System immunology, Dura Mater cytology, Lymphopoiesis, Meninges cytology, Meninges immunology, Skull anatomy & histology

Abstract

The meninges contain adaptive immune cells that provide immunosurveillance of the central nervous system (CNS). These cells are thought to derive from the systemic circulation. Through single-cell analyses, confocal imaging, bone marrow chimeras, and parabiosis experiments, we show that meningeal B cells derive locally from the calvaria, which harbors a bone marrow niche for hematopoiesis. B cells reach the meninges from the calvaria through specialized vascular connections. This calvarial-meningeal path of B cell development may provide the CNS with a constant supply of B cells educated by CNS antigens. Conversely, we show that a subset of antigen-experienced B cells that populate the meninges in aging mice are blood-borne. These results identify a private source for meningeal B cells, which may help maintain immune privilege within the CNS., (Copyright © 2021 The Authors, some rights reserved; exclusive licensee American Association for the Advancement of Science. No claim to original U.S. Government Works.)

Published

2021

9. Mechanical Properties of the Cranial Meninges: A Systematic Review.

Author

Walsh DR, Zhou Z, Li X, Kearns J, Newport DT, and Mulvihill JJE

Subjects

Animals, Arachnoid cytology, Brain cytology, Brain physiology, Dura Mater cytology, Humans, Meninges cytology, Meninges physiology, Pia Mater cytology, Arachnoid physiology, Biomechanical Phenomena physiology, Dura Mater physiology, Pia Mater physiology

Abstract

The meninges are membranous tissues that are pivotal in maintaining homeostasis of the central nervous system. Despite the importance of the cranial meninges in nervous system physiology and in head injury mechanics, our knowledge of the tissues' mechanical behavior and structural composition is limited. This systematic review analyzes the existing literature on the mechanical properties of the meningeal tissues. Publications were identified from a search of Scopus, Academic Search Complete, and Web of Science and screened for eligibility according to Preferred Reporting Items for Systematic Reviews and Meta-Analyses guidelines. The review details the wide range of testing techniques employed to date and the significant variability in the observed experimental findings. Our findings identify many gaps in the current literature that can serve as a guide for future work for meningeal mechanics investigators. The review identifies no peer-reviewed mechanical data on the falx and tentorium tissues, both of which have been identified as key structures in influencing brain injury mechanics. A dearth of mechanical data for the pia-arachnoid complex also was identified (no experimental mechanics studies on the human pia-arachnoid complex were identified), which is desirable for biofidelic modeling of human head injuries. Finally, this review provides recommendations on how experiments can be conducted to allow for standardization of test methodologies, enabling simplified comparisons and conclusions on meningeal mechanics.

Published

2021

10. Tissue-nonspecific alkaline phosphatase promotes the osteogenic differentiation of osteoprogenitor cells.

Author

Nakamura T, Nakamura-Takahashi A, Kasahara M, Yamaguchi A, and Azuma T

Subjects

Animals, Core Binding Factor Alpha 1 Subunit metabolism, Dura Mater cytology, Extracellular Matrix Proteins metabolism, Levamisole pharmacology, Mice, Inbred C57BL, Osteoblasts cytology, Osteoblasts drug effects, Osteoblasts metabolism, Phosphates pharmacology, Skull cytology, Alkaline Phosphatase metabolism, Cell Differentiation drug effects, Osteogenesis drug effects, Stem Cells cytology, Stem Cells metabolism

Abstract

Tissue-nonspecific alkaline phosphatase (TNAP) is expressed in the calcification sites of the skeletal tissue. It promotes hydroxyapatite crystal formation by degrading inorganic pyrophosphate (PP i ) and increasing inorganic phosphate (P i ) concentration. However, abnormalities in Alpl -/- mouse-derived osteoblasts are poorly understood, and the involvement of TNAP in osteoblast differentiation remains unclear. Therefore, in this study, we aimed to investigate the precise role of TNAP in osteoblast differentiation. TNAP inhibition by levamisole, a reversible TNAP inhibitor, suppressed the expression of osteoblast differentiation marker genes in wild-type osteoblastic cells. Alpl overexpression increased the expression of master osteoblast transcription factor genes runt-related transcription factor 2 (Runx2) and Sp7 and the mature osteoblast and osteocyte marker genes, bone γ-carboxyglutamate protein 2 (Bglap2) and dentin matrix protein 1 (Dmp1), respectively in Alpl-deficient osteoblastic cells. TNAP regulated Runx2 expression, which in turn regulated the expression of all other osteoblast markers, except Dmp1. Dmp1 expression was independent of RUNX2 but was dependent on extracellular P i concentration in Runx2-deficient osteogenic cells. These results suggest that TNAP functions as an osteogenic differentiation regulator either by regulating Runx2 expression or by controlling extracellular P i concentration., (Copyright © 2020 Elsevier Inc. All rights reserved.)

Published

2020

11. The Flavor Enhancer Maltol Increases Pigment Aggregation in Dermal and Neural Melanophores in Xenopus laevis Tadpoles.

Author

Dahora LI, Fitzgerald A, Emanuel M, Baiges AF, Husain Z, and Thompson CK

Subjects

Animals, Dose-Response Relationship, Drug, Dura Mater cytology, Dura Mater metabolism, Flavoring Agents metabolism, Gene Expression drug effects, Larva genetics, Larva metabolism, Larva radiation effects, Melanophores metabolism, Melatonin metabolism, Melatonin pharmacology, Pigmentation drug effects, Pyrones metabolism, Skin cytology, Skin metabolism, Toxicity Tests, Ultraviolet Rays, Xenopus laevis, Dura Mater drug effects, Flavoring Agents toxicity, Larva drug effects, Melanophores drug effects, Pigments, Biological metabolism, Pyrones toxicity, Skin drug effects

Abstract

Melanophores are pigmented cells that change the distribution of melanosomes, enabling animals to appear lighter or darker for camouflage, thermoregulation, and protection from ultraviolet radiation. A complex series of hormonal and neural mechanisms regulates melanophore pigment distribution, making these dynamic cells a valuable tool to screen toxicants as they rapidly respond to changes in the environment. We found that maltol, a naturally occurring flavor enhancer and fragrance agent, induces melanophore pigment aggregation in a dose-dependent manner in Xenopus laevis tadpoles. To determine if maltol affects camouflage adaptation, we placed tadpoles into maltol baths situated over either a white or a black background. Maltol induced pigment aggregation in a similar dose-dependent pattern regardless of background color. We also tested how maltol treatment compares to melatonin treatment and found that the degree of pigment aggregation induced by maltol is similar to treatment with melatonin but that maltol induces over a much longer time course. Last, maltol had no effect on mRNA expression in the brain of genes that regulate camouflage-related pigment aggregation. The present results suggest that maltol does not exert its effects via the camouflage adaptation mechanism or via melatonin-related mechanisms. These results are the first to identify a putative toxicological effect of maltol exposure in vivo and rule out several mechanisms by which maltol may exert its effects on pigment aggregation. Environ Toxicol Chem 2020;39:381-395. © 2019 SETAC., (© 2019 SETAC.)

Published

2020

12. In Vivo Evaluation of Novel PLA/PCL Polymeric Patch in Rats for Potential Spina Bifida Coverage.

Author

Oria M, Tatu RR, Lin CY, and Peiro JL

Subjects

Animals, Rats, Astrocytes pathology, Disease Models, Animal, Dura Mater cytology, Dura Mater pathology, Dura Mater surgery, Gliosis diagnosis, Gliosis etiology, Gliosis pathology, Laminectomy, Materials Testing, Postoperative Complications diagnosis, Postoperative Complications etiology, Neurosurgical Procedures adverse effects, Neurosurgical Procedures instrumentation, Polyesters adverse effects, Prostheses and Implants adverse effects, Spinal Dysraphism surgery

Abstract

Background: Current therapeutic materials for spina bifida repair showed a limited number of options in the market, and none of them have all the requirements as the ideal patch. In fact, sometimes the surgical procedures pose substantial challenges using different patches to fully cover the spina bifida lesion. For this purpose, a tailored patch made of poly (L-lactic acid) and poly (ε-caprolactone) blend was designed and validated in vitro to accomplish all these requirements but was never tested in vivo., Material and Methods: In our present study, the designed patch was analyzed in terms of rejection from the animal when implanted subcutaneously and as a dural substitute in the spinal cord. Inflammatory reaction (Iba1), astrogliosis (GFAP), was analyzed and functional interaction with spinal cord tissue assessing the (%motor-evoked potentials /compound motor action potential) by electrophysiology., Results: No evidence of adverse or inflammatory reactions was observed in both models of subcutaneous implantation, neither in the neural tissue as a dural substitute. No signs of astrogliosis in the neural tissue were observed, and no functional alteration with improvement of the motor-evoked potential's amplitude was detected after 4 wk of implantation as a dural substitute in the rat spinal cord., Conclusions: Designed patch used as a dural substitute will apparently not produce inflammation, scar formation, or tethering cord and not induce any adverse effect on regular functions of the spinal cord. Further studies are needed to evaluate potential improvements of this novel polymeric patch in the spinal cord regeneration using spina bifida models., (Copyright © 2019. Published by Elsevier Inc.)

Published

2019

13. Mechanical and morphological description of human acellular dura mater as a scaffold for surgical reconstruction.

Author

J Z, B O, M S, G ST, and N H

Subjects

Adolescent, Adult, Aged, Aged, 80 and over, Biomechanical Phenomena, Child, Dura Mater cytology, Female, Humans, Male, Materials Testing, Middle Aged, Young Adult, Mechanical Phenomena, Plastic Surgery Procedures methods, Tissue Scaffolds

Abstract

As native human dura mater has been successfully used as a transplant, the acellular dura mater scaffold is a promising material for the same purpose, that is less prone to transplant rejection. A detailed knowledge of the dura material properties may also aid to tissue engineer customized scaffolds mechanically mimicking the healthy natural condition. Both native and acellular dura have to date not been satisfactorily described concerning their load-deformation properties and the morphology related to scaffold mechanics. We investigated the tensile properties of 18 acellular human dura samples and compared these to the values of 18 matched native counterparts of the same donors. A highly standardized approach in material testing was used with coupled image correlation, involving 3D-printed clamps and fixtures, and adaptation of the tissue water content. The tensile parameters of acellular dura appeared to differ only minutely from the native condition. The removal of cells appeared not to vastly influence the biomechanics of dura. Lower values of the elastic modulus (36 vs. 74 MPa, p < 0.01) and ultimate tensile strength (4 vs. 7 MPa, p = 0.05) of acellular dura compared to the native counterparts were likely the consequence of tissue swelling related to the acellularization procedure. Collagens and proteoglycans remained intact in the acellular state, whereas glycosaminoglycans appeared to decrease. Fibronectin and elastic fibres were exposed by the removal of cells. Consequently, seeding these acellular scaffolds with cells appears not to be necessary from a biomechanical perspective., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2019

14. Non-Trigeminal Nociceptive Innervation of the Posterior Dura: Implications to Occipital Headache.

Author

Noseda R, Melo-Carrillo A, Nir RR, Strassman AM, and Burstein R

Subjects

Animals, Cervical Cord physiology, Male, Neural Pathways cytology, Neural Pathways physiology, Neuroanatomical Tract-Tracing Techniques, Rats, Sprague-Dawley, Dura Mater cytology, Dura Mater physiology, Ganglia, Spinal cytology, Ganglia, Spinal physiology, Headache physiopathology, Neurons cytology, Neurons physiology, Nociceptors physiology

Abstract

Current understanding of the origin of occipital headache falls short of distinguishing between cause and effect. Most preclinical studies involving trigeminovascular neurons sample neurons that are responsive to stimulation of dural areas in the anterior 2/3 of the cranium and the periorbital skin. Hypothesizing that occipital headache may involve activation of meningeal nociceptors that innervate the posterior ⅓ of the dura, we sought to map the origin and course of meningeal nociceptors that innervate the posterior dura overlying the cerebellum. Using AAV-GFP tracing and single-unit recording techniques in male rats, we found that neurons in C2-C3 DRGs innervate the dura of the posterior fossa; that nearly half originate in DRG neurons containing CGRP and TRPV1; that nerve bundles traverse suboccipital muscles before entering the cranium through bony canals and large foramens; that central neurons receiving nociceptive information from the posterior dura are located in C2-C4 spinal cord and that their cutaneous and muscle receptive fields are found around the ears, occipital skin and neck muscles; and that administration of inflammatory mediators to their dural receptive field, sensitize their responses to stimulation of the posterior dura, peri-occipital skin and neck muscles. These findings lend rationale for the common practice of attempting to alleviate migraine headaches by targeting the greater and lesser occipital nerves with anesthetics. The findings also raise the possibility that such procedures may be more beneficial for alleviating occipital than non-occipital headaches and that occipital migraines may be associated more closely with cerebellar abnormalities than in non-occipital migraines. SIGNIFICANCE STATEMENT Occipital headaches are common in both migraine and non-migraine headaches. Historically, two distinct scenarios have been proposed for such headaches; the first suggests that the headaches are caused by spasm or tension of scalp, shoulders, and neck muscles inserted in the occipital region, whereas the second suggests that these headaches are initiated by activation of meningeal nociceptors. The current study shows that the posterior dura overlying the cerebellum is innervated by cervicovascular neurons in C2 DRG whose axons reach the posterior dura through multiple intracranial and extracranial pathways, and sensitization of central cervicovascular neurons from the posterior dura can result in hyper-responsiveness to stimulation of neck muscles. The findings suggest that the origin of occipital and frontal migraine may differ., (Copyright © 2019 the authors 0270-6474/19/391867-14$15.00/0.)

Published

2019

15. Inflammation by activated macrophage-like THP-1 cells increases human dura mater cell adhesion with alteration of integrin α 2 β 1 and matrix metalloproteinase.

Author

Chong K, Kwon WK, Kim JH, Park YK, Yoon W, Kim JH, Kwon TH, and Moon HJ

Subjects

Adult, Aged, Coculture Techniques, Collagen Type I physiology, Collagen Type IV physiology, Dura Mater enzymology, Dura Mater physiopathology, Female, Humans, Integrin alpha2beta1 physiology, Male, Middle Aged, Primary Cell Culture, THP-1 Cells, Cell Adhesion, Dura Mater cytology, Extracellular Matrix physiology, Inflammation physiopathology, Matrix Metalloproteinases metabolism

Abstract

This study was designed to investigate (i) extracellular matrix to specify adhesive substrates to human dura mater cell (hDMC); (ii) the alteration on adhesion-related molecules in hDMC; and (iii) secreted matrix metalloproteinases (MMPs) linked with extracellular matrix remodeling after exposure to inflammation. The hDMC was cultured from human dura mater tissue, and the studies were performed with hDMC after co-culturing with macrophage like THP-1 cells (Mϕ). The adhesion of co-cultured hDMC through collagen I increased 6.4-fold and through collagen IV increased 5.0-fold compared with the adhesion of naïve cells (p < 0.001). Integrin subtype α 2 β 1 expression was increased 6.3-fold (p < 0.001) and α 1 expression was decreased 2.0-fold (p < 0.001) in the co-cultured cells compared with the naïve cells. Co-culturing induced significant increases in MMP-1 (13.9-fold, p < 0.01), MMP-3 (7.6-fold, p < 0.01), and VEGF (VEGF: 3.8-fold, p < 0.05) expression and decreases in MMP-9 (0.1-fold, p < 0.01) compared with the sum of naïve hDMC and Mϕ values. Increased hDMC adhesion under inflammatory conditions is caused by an increased cellular affinity for collagen I and IV mediated by increased hDMC levels of integrin subtype α 2 β 1 and environmental MMP-1, -3 and decreased MMP-9. Selective integrin subtype α 2 β 1 inhibition assay showed 37.8% and 35.7% reduction in adhesion of co-cultured hDMC to collagen I (p < 0.001) and IV (p = 0.057), respectively. The present study provides insight into the pathological conditions related to dura mater adhesion in inflammation. © 2018 Orthopaedic Research Society. Published by Wiley Periodicals, Inc. J Orthop Res 9999:1-11, 2019., (© 2018 Orthopaedic Research Society. Published by Wiley Periodicals, Inc.)

Published

2019

16. Dural Cells Release Factors Which Promote Cancer Cell Malignancy and Induce Immunosuppressive Markers in Bone Marrow Myeloid Cells.

Author

Szerlip NJ, Calinescu A, Smith E, Tagett R, Clines KL, Moon HH, Taichman RS, Van Poznak CH, and Clines GA

Subjects

Animals, Bone Marrow Cells metabolism, Cell Proliferation, Cells, Cultured, Culture Media, Conditioned pharmacology, Cytokines pharmacology, Dura Mater metabolism, Humans, Male, Mice, Neoplasm Metastasis pathology, Cytokines metabolism, Dura Mater cytology, Fibroblasts metabolism, Myeloid Cells metabolism, Neoplasms pathology

Abstract

Background: Thirty per cent of cancer patients develop spine metastases with a substantial number leading to spinal cord compression and neurological deficits. Many demonstrate a propensity toward metastasis to the posterior third of the vertebral body. The dura, the outer layer of the meninges, lies in intimate contact with the posterior border of the vertebral body and has been shown to influence adjacent bone. The effects of the dura on bone marrow and cancer cells have not been examined. Understanding the biology of spinal metastasis will provide insights into mechanisms of cancer growth and allow for new treatment strategies., Objective: To examine the extent to which dura influences bone marrow/tumor cell metastatic characteristics., Methods: Dura conditioned media (DCM) from primary dura was examined for the ability to stimulate tumor cell proliferation/invasion and to alter bone marrow cell populations. RNA sequencing of dural fibroblasts was performed to examine expression of cytokines and growth factors., Results: DCM induced a significant increase in invasion and proliferation of multiple tumor cell lines, and of patient-derived primary spinal metastatic cells. DCM also increased the proliferation of bone marrow myeloid cells, inducing expression of immunosuppressive markers. RNA sequencing of dural fibroblasts demonstrated abundant expression of cytokines and growth factors involved in cancer/immune pathways., Conclusion: Factors released by primary dural cells induce proliferation of tumor cells and alter bone marrow to create a fertile environment for tumor growth. The dura therefore may play an important role in the increased incidence of metastases to adjacent bone.

Published

2018

17. Modulation of tetrodotoxin-resistant Na + channels by amitriptyline in dural afferent neurons.

Author

Kang IS, Cho JH, Lee MG, and Jang IS

Subjects

Amitriptyline therapeutic use, Animals, Antidepressive Agents, Tricyclic therapeutic use, Dura Mater cytology, Dura Mater metabolism, Male, Membrane Potentials drug effects, Migraine Disorders pathology, Nociceptors metabolism, Patch-Clamp Techniques, Rats, Rats, Sprague-Dawley, Sodium Channel Blockers pharmacology, Sodium Channels metabolism, Tetrodotoxin pharmacology, Amitriptyline pharmacology, Antidepressive Agents, Tricyclic pharmacology, Migraine Disorders drug therapy, Nociceptors drug effects, Sodium Channels drug effects

Abstract

Migraine is characterized by recurrent and disabling headaches; therefore, several drugs have been widely prescribed to prevent acute migraine attacks. Amitriptyline, a tricyclic antidepressant, is among the most commonly administered. It is poorly known, however, whether amitriptyline modulates the excitability of dural afferent neurons that transmit pain signals from the dura mater. In this study, the effects of amitriptyline on tetrodotoxin-resistant (TTX-R) Na + channels were examined in acutely isolated rat dural afferent neurons, which were identified by the fluorescent dye DiI. The TTX-R Na + currents (I Na ) were recorded from medium-sized DiI-positive neurons using a whole-cell patch clamp technique. Amitriptyline (3 μM) slightly reduced the peak component of transient I Na and induced a marked decrease in the steady-state component of transient TTX-R I Na , as well as in the slow ramp-induced TTX-R I Na . Our findings suggest that amitriptyline specifically inhibits persistent Na + currents mediated by TTX-R Na + channels. While amitriptyline had minor effects on voltage-activation/inactivation, it increased the extent of the use-dependent inhibition of TTX-R Na + channels. Amitriptyline also affected the inactivation kinetics of TTX-R Na + channels by significantly accelerating the inactivation of TTX-R Na + channels and slowing the subsequent recovery. Amitriptyline decreased the number of action potentials by increasing the threshold for their generation. In conclusion, the amitriptyline-mediated diverse modulation of TTX-R Na + channels would be, at least in part, responsible for its prophylactic efficacy for migraine attacks., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published

2018

18. Activation of pial and dural macrophages and dendritic cells by cortical spreading depression.

Author

Schain AJ, Melo-Carrillo A, Borsook D, Grutzendler J, Strassman AM, and Burstein R

Subjects

Animals, Dendritic Cells chemistry, Dura Mater chemistry, Dura Mater cytology, Female, Macrophages chemistry, Male, Mice, Mice, Inbred C57BL, Mice, Transgenic, Pia Mater chemistry, Pia Mater cytology, TRPV Cation Channels chemistry, TRPV Cation Channels physiology, Cortical Spreading Depression physiology, Dendritic Cells physiology, Dura Mater physiology, Macrophages physiology, Pia Mater physiology

Abstract

Objective: Cortical spreading depression (CSD) has long been implicated in migraine attacks with aura. The process by which CSD, a cortical event that occurs within the blood-brain barrier (BBB), results in nociceptor activation outside the BBB is likely mediated by multiple molecules and cells. The objective of this study was to determine whether CSD activates immune cells inside the BBB (pia), outside the BBB (dura), or in both, and if so, when., Methods: Investigating cellular events in the meninges shortly after CSD, we used in vivo two-photon imaging to identify changes in macrophages and dendritic cells (DCs) that reside in the pia, arachnoid, and dura and their anatomical relationship to TRPV1 axons., Results: We found that activated meningeal macrophages retract their processes and become circular, and that activated meningeal DCs stop migrating. We found that CSD activates pial macrophages instantaneously, pial, subarachnoid, and dural DCs 6-12 minutes later, and dural macrophages 20 minutes later. Dural macrophages and DCs can appear in close proximity to TRPV1-positive axons., Interpretation: The findings suggest that activation of pial macrophages may be more relevant to cases where aura and migraine begin simultaneously, that activation of dural macrophages may be more relevant to cases where headache begins 20 to 30 minutes after aura, and that activation of dural macrophages may be mediated by activation of migratory DCs in the subarachnoid space and dura. The anatomical relationship between TRPV1-positive meningeal nociceptors, and dural macrophages and DCs supports a role for these immune cells in the modulation of head pain. Ann Neurol 2018;83:508-521., (© 2018 American Neurological Association.)

Published

2018

19. The posterior epidural ligament in the thoracic region: a cadaveric and histological study.

Author

Rimmer CT and Adds PJ

Subjects

Aged, Aged, 80 and over, Cadaver, Dissection, Female, Humans, Ligamentum Flavum anatomy & histology, Ligamentum Flavum cytology, Male, Dura Mater anatomy & histology, Dura Mater cytology, Ligaments anatomy & histology, Ligaments cytology, Thorax anatomy & histology

Abstract

The existence of posterior epidural ligaments (PEL) has been established in the lumbar region, but they have hitherto not been shown to exist in the thoracic vertebral column. Their identification is of clinical significance in respect to incidental durotomy and the circulation of cerebrospinal fluid (CSF). Fourteen thoracic spine sections were dissected by cutting through the intervertebral disc and separating the ligamentum flavum from the vertebra above. The dural sheath was gently retracted anteriorly to identify macroscopic connections between the ligamentum flavum and the dura. Macroscopic connections observed were dissected out, retaining some dural sheath and ligamentum flavum. Histological staining with haematoxylin and eosin and Miller's elastin stain was used to investigate cellular connections. Thoracic PELs were positively identified in 5 of the 14 cadavers (35.7%). Histology showed similarities between the thoracic and lumbar PELs. Fifteen separate PELs were identified within these five thoracic sections. The thoracic PEL has sufficient tensile strength to present a risk to the integrity of the dural sheath during surgery, and surgeons should be aware of these connections when operating on the thoracic spine. PELs may also contribute to the circulation of CSF in the spinal subarachnoid space.

Published

2018

20. Effects of Nigella sativa seeds and certain species of fungi extracts on number and activation of dural mast cells in rats.

Author

Kilinc E, Dagistan Y, Kotan B, and Cetinkaya A

Subjects

Analgesics isolation & purification, Animals, Anti-Inflammatory Agents isolation & purification, Dura Mater cytology, Male, Mast Cells immunology, Mast Cells microbiology, Phytotherapy, Plant Extracts isolation & purification, Plants, Medicinal, Rats, Wistar, Tricholoma chemistry, p-Methoxy-N-methylphenethylamine pharmacology, Analgesics pharmacology, Anti-Inflammatory Agents pharmacology, Cell Degranulation drug effects, Fungi chemistry, Mast Cells drug effects, Nigella sativa chemistry, Plant Extracts pharmacology, Seeds chemistry

Abstract

In this study, we aimed to investigate the effects of Nigella sativa seeds and certain species of fungi extracts on the number and degranulation states of dural mast cells in rats. Rats were fed ad libitum with normal tap water or tap water with extract of N. sativa seed, Ramaria condensata, Lactarius salmonicolor, Lactarius piperatus, and Tricholoma terreum for 3 days. Mast cells in dura mater were counted and evaluated in terms of granulation and degranulation states. Compound 48/80, a mast cell degranulating agent, and T. terreum significantly increased the percent of degranulated mast cells in dura mater, respectively (p < 0.01 and p < 0.05). Moreover, T. terreum causes a significant increase in the total number of mast cells (p < 0.05). N. sativa significantly inhibited mast cell degranulation induced by both the compound 48/80 and T. terreum (p < 0.05), and significantly decreased the mast cell numbers increased by T. terreum (p < 0.05). Our results suggested that T. terreum following ingestion can contribute to headaches like migraine via dural mast cell degranulation and N. sativa may be able to exert analgesic and anti-inflammatory effects by stabilizing dural mast cells. However, investigation is needed to determine the ingredients of N. sativa that may be responsible for these beneficial effects.

Published

2017

21. Monosodium glutamate alters the response properties of rat trigeminovascular neurons through activation of peripheral NMDA receptors.

Author

O'Brien M and Cairns BE

Subjects

Action Potentials drug effects, Animals, Dura Mater blood supply, Dura Mater cytology, Dura Mater metabolism, Excitatory Amino Acid Antagonists pharmacology, Excitatory Amino Acid Transporter 2 metabolism, Female, Male, Rats, Sprague-Dawley, Receptors, N-Methyl-D-Aspartate antagonists & inhibitors, Sensory Receptor Cells cytology, Sensory Receptor Cells metabolism, Sensory Thresholds drug effects, Sex Characteristics, Tegmentum Mesencephali cytology, Tegmentum Mesencephali metabolism, Touch drug effects, Touch physiology, Valine analogs & derivatives, Valine pharmacology, Vasodilation drug effects, Vasodilation physiology, Dura Mater drug effects, Receptors, N-Methyl-D-Aspartate metabolism, Sensory Receptor Cells drug effects, Sodium Glutamate pharmacology, Tegmentum Mesencephali drug effects, Vasodilator Agents pharmacology

Abstract

Ingestion of monosodium glutamate (MSG) has been shown to cause headaches in healthy individuals and trigger migraine-like headaches in migraine sufferers. We combined immunohistochemistry, in vivo electrophysiology, and laser Doppler recordings of dural vasculature to investigate the effect of systemic administration of MSG on the trigeminovascular pathway. Immunohistochemical analysis confirmed the expression of NMDA receptors on nerve fibers innervating dural blood vessels and excitatory amino acid transporter 2 on dural blood vessels. Systemic administration of MSG (50mg/kg) evoked an increase in ongoing discharge in 5/6 spinal trigeminal subnucleus caudalis (SpVc) neurons with dural input recorded from male and female rats, respectively, as well as lowering their mechanical activation threshold. There were no sex-related differences in these effects of MSG. Neuronal discharge and mechanical sensitization were significantly attenuated by co-injection with the peripherally restricted NMDA receptor antagonist (2R)-amino-5-phosphonovaleric acid (APV) in both sexes. Systemic administration of MSG induced a 24.5% and 20.6% increase in dural flux in male and female rats, respectively. These results suggest that MSG-induced headache is mediated by the activation of peripheral NMDA receptors and subsequent dural vasodilation. Peripheral NMDA receptors are a potential target for the development of new drugs to treat headaches., (Copyright © 2016 IBRO. Published by Elsevier Ltd. All rights reserved.)

Published

2016

22. Immunohistochemical localization of the calcitonin gene-related peptide binding site in the primate trigeminovascular system using functional antagonist antibodies.

Author

Miller S, Liu H, Warfvinge K, Shi L, Dovlatyan M, Xu C, and Edvinsson L

Subjects

Aged, Animals, Antibodies, Binding Sites, Blotting, Western, Calcitonin Receptor-Like Protein immunology, Calcitonin Receptor-Like Protein metabolism, Cell Line, Tumor, Dura Mater blood supply, Dura Mater cytology, Dura Mater metabolism, Female, Humans, Immunohistochemistry, Macaca fascicularis, Male, Meningeal Arteries cytology, Middle Aged, Migraine Disorders metabolism, Muscle, Smooth, Vascular cytology, Muscle, Smooth, Vascular metabolism, Myocytes, Smooth Muscle cytology, Neuroglia cytology, Neurons cytology, Receptor Activity-Modifying Protein 1 immunology, Receptor Activity-Modifying Protein 1 metabolism, Receptors, Calcitonin Gene-Related Peptide immunology, Trigeminal Ganglion cytology, Meningeal Arteries metabolism, Myocytes, Smooth Muscle metabolism, Neuroglia metabolism, Neurons metabolism, Receptors, Calcitonin Gene-Related Peptide metabolism, Trigeminal Ganglion metabolism

Abstract

Calcitonin gene-related peptide (CGRP) is a potent vasodilator and a neuromodulator implicated in the pathophysiology of migraine. It binds to the extracellular domains of calcitonin receptor-like receptor (CLR) and receptor activity-modifying protein (RAMP) 1 that together form the CGRP receptor. Antagonist antibodies against CGRP and its binding site at the receptor are clinically effective in preventing migraine attacks. The blood-brain barrier penetration of these antagonist antibodies is limited, suggesting that a potential peripheral site of action is sufficient to prevent migraine attacks. To further understand the sites of CGRP-mediated signaling in migraine, we used immunohistochemical staining with recently developed antagonist antibodies specifically recognizing a fusion protein of the extracellular domains of RAMP1 and CLR that comprise the CGRP binding pocket at the CGRP receptor in monkey and man. We confirmed binding of the antagonist antibodies to human vascular smooth muscle cells (VSMCs) of dural meningeal arteries and neurons in the trigeminal ganglion, both of which are likely sites of action for therapeutic antibodies in migraine patients. We further used one of these antibodies for detailed mapping on cynomolgus monkey tissue and found antagonist antibody binding sites at multiple levels in the trigeminovascular system: in the dura mater VSMCs, in neurons and satellite glial cells in the trigeminal ganglion, and in neurons in the spinal trigeminal nucleus caudalis. These data reinforce and clarify our understanding of CGRP receptor localization in a pattern consistent with a role for CGRP receptors in trigeminal sensitization and migraine pathology., (Copyright © 2016 IBRO. Published by Elsevier Ltd. All rights reserved.)

Published

2016

23. The Transdural Course of Radicular Spinal Cord Veins--A Microangiographical and Microscopical Study.

Author

Thron A, Krings T, Otto J, Mull M, and Schroeder JM

Subjects

Humans, Spinal Cord cytology, Spinal Cord diagnostic imaging, Dura Mater cytology, Dura Mater diagnostic imaging, Phlebography methods, Spinal Cord blood supply, Veins cytology

Abstract

Purpose: This study focuses on the following questions: What are the morphological features at the transdural course of radiculomedullary veins? How are these short transdural segments that may harbour pathological arteriovenous shunts connected to the internal vertebral venous plexus? Is the conception of a reflux-impeding mechanism at the transdural segment indispensable and convincing?, Methods: A total of 102 radiculospinal veins were studied microscopically at various levels of the spinal canal using serial paraffin and semi-thin sections. In addition, 26 vessels were investigated microangiographically following orthograde (12) or attempted retrograde (14) opacification of the intradural venous segment with barium sulphate. After paraplast-embedding, contact-microradiographs were taken using high-resolution spectroscopic plates., Results: At their transdural course, the veins showed narrowing of their lumen accompanied by changes in the vessel wall composition and a tortuous course. Two structurally distinct arrangements of the transdural segment could be identified: A slit type was seen in 60% of the veins studied and a bulge- or nodular type was seen in 35% of the veins. In total, 5% of cases could not be assigned to either one of these types. Reflux to radicular veins from the outside of the dura mater could be produced in 2 out of 14 specimens. The extradural venous plexus, which primarily receives the radicular vein, was composed more frequently of lacunar spaces rather than plexiform blood vessel convolutions. Rare observations were fibrotic, blind ending radiculomedullary veins and continuation of a distinct venous blood vessel after crossing the dura., Conclusions: Reflux from the epidural plexus to radicular veins is not reliably stopped at the dural level and possibly physiological. Different arrangements of the transdural course of the veins appear to be at least appropriate to modulate flow. The purpose for two different types of radicular vein exit is unclear. The clinical impact of disturbed reflux-control is uncertain, which is in stark contrast to the severe consequences resulting from dural arteriovenous shunts. The functional role of the probably predominant epidural venous plexus for the spinal cord blood circulation remains poorly understood.

Published

2015

24. Cell Therapy: Engineering and Manufacture of Pluripotent Cells.

Author

Guinto G, Zepeda E, and Londoño D

Subjects

Animals, Humans, Male, Dura Mater cytology, Induced Pluripotent Stem Cells, Neural Stem Cells, Ventriculoperitoneal Shunt

Published

2015

25. Efficient Generation of Induced Pluripotent Stem and Neural Progenitor Cells From Acutely Harvested Dura Mater Obtained During Ventriculoperitoneal Shunt Surgery.

Author

Cary WA, Hori CN, Pham MT, Nacey CA, McGee JL, Hamou M, Berman RF, Bauer G, Nolta JA, and Waldau B

Subjects

Animals, Cell Differentiation, Cellular Reprogramming, Clone Cells, Cognition Disorders etiology, Dura Mater surgery, Fibroblasts, Humans, Hydrocephalus, Normal Pressure surgery, Karyotyping, Male, Mice, Middle Aged, Sendai virus, Teratoma pathology, Transcription Factors metabolism, Dura Mater cytology, Induced Pluripotent Stem Cells metabolism, Neural Stem Cells metabolism, Ventriculoperitoneal Shunt

Abstract

Background: The dura mater can be easily biopsied during most cranial neurosurgical operations. We describe a protocol that allows for robust generation of induced pluripotent stem cells (iPSCs) and neural progenitors from acutely harvested dura mater., Objective: To generate iPSCs and neural progenitor cells from dura mater obtained during ventriculoperitoneal shunt surgery., Methods: Dura was obtained during ventriculoperitoneal shunt surgery for normal pressure hydrocephalus from a 60-year-old patient with severe cognitive impairment. Fibroblasts were isolated from the dural matrix and transduced with nonintegrating Sendai virus for iPSC induction. A subset of successfully generated iPSC clones underwent immunocytochemical analysis, teratoma assay, karyotyping, and targeted neural differentiation., Results: Eleven iPSC clones were obtained from the transduction of an estimated 600,000 dural fibroblasts after 3 passages. Three clones underwent immunocytochemical analysis and were shown to express the transcription factors OCT-4, SOX2, and the embryonic cell markers SSEA-4, TRA-1-60, and Nanog. Two clones were tested for pluripotency and formed teratomas at the injection site in immunodeficient mice. Three clones underwent chromosomal analysis and were found to have a normal metaphase spread and karyotype. One clone underwent targeted neural differentiation and formed neural rosettes as well as TuJ1/SOX1-positive neural progenitor cells., Conclusions: IPSCs and neural progenitor cells can be efficiently derived from the dura of patients who need to undergo cranial neurosurgical operations. IPSCs were obtained with a nonintegrating virus and exhibited a normal karyotype, making them candidates for future autotransplantation after targeted differentiation to treat functional deficits., (Copyright © 2015. Published by Elsevier Inc.)

Published

2015

26. Sex-, Stress-, and Sympathetic Post-Ganglionic Neuron-Dependent Changes in the Expression of Pro- and Anti-Inflammatory Mediators in Rat Dural Immune Cells.

Author

McIlvried LA, Borghesi LA, and Gold MS

Subjects

Animals, Dura Mater cytology, Dura Mater metabolism, Female, Inflammation metabolism, Male, RNA, Messenger metabolism, Rats, Rats, Sprague-Dawley, Sex Factors, Dura Mater immunology, Inflammation immunology, Inflammation Mediators metabolism, Migraine Disorders immunology, Stress, Psychological immunology, Sympathetic Fibers, Postganglionic immunology

Abstract

Background: Migraine attacks are associated with sterile inflammation of the dura. Immune cells are a primary source of inflammatory mediators, and we therefore sought to further explore the link between dural immune cells and migraine., Objective: Based on the observations that migraine is more common in women than in men, stress is the most common trigger for a migraine attack, and sympathetic post-ganglionic innervation of the dura enables local control of dural immune cells, we hypothesized that stress shifts the balance of inflammatory mediator expression in dural immune cells toward those that trigger a migraine attack, where these changes are larger in females and dependent, at least in part, on sympathetic post-ganglionic innervation of the dura. Our objective was to test this hypothesis., Methods: Dura were obtained from naïve or stressed, intact or surgically sympathectomized, adult male and female rats. Dura were assessed immediately or 24 hours after termination of 4 continuous days of unpredictable, mild stressors. Following enzymatic digestion of each dura, myeloid and lymphoid-derived dural immune cells were isolated by fluorescence-activated cell sorting for semi-quantitative polymerase chain reaction analysis., Results: In myeloid-derived dural immune cells, there was an increase in pro-inflammatory mediator mRNA following stress, particularly in females, which remained elevated with a 24-hour delay after stress. There was a stress-induced decrease in anti-inflammatory mediator mRNA immediately after stress in females, but not males. The stress-induced changes were attenuated in sympathectomized females. In lymphoid-derived dural immune cells, there was a persistent increase in pro-inflammatory mediator mRNA following stress, particularly in females. A stress-induced increase in anti-inflammatory mediator mRNA was also observed in both males and females, and was further attenuated in sympathectomized females., Conclusions: Consistent with our hypothesis, there is a stress-induced shift in the balance of pro- and anti-inflammatory mediator expression in dural immune cells that is more pronounced in females, and is dependent, at least in part, on sympathetic post-ganglionic innervation in females. This shift in the balance of inflammatory mediator expression may not only play an important role in triggering migraine attacks, but also suggests it may be possible, if not necessary, to employ different strategies to most effectively treat migraine in men and women., (© 2015 American Headache Society.)

Published

2015

27. Vasoactive Intestinal peptide modulates c-Fos activity in the trigeminal nucleus and dura mater mast cells in sympathectomized rats.

Author

Kilinc E, Firat T, Tore F, Kiyan A, Kukner A, and Tunçel N

Subjects

Animals, Male, Rats, Rats, Sprague-Dawley, Statistics, Nonparametric, Trigeminal Nuclei metabolism, Dura Mater cytology, Mast Cells drug effects, Oncogene Proteins v-fos metabolism, Sympathectomy, Trigeminal Nuclei drug effects, Vasoactive Intestinal Peptide pharmacology

Abstract

Neurogenic inflammation in the dura mater caused by trigeminal nociceptive activation has been implicated in the pathophysiology of migraine. Vasoactive intestinal polypeptide (VIP) is a powerful neuroprotective neuropeptide that can modulate mast cell behavior. Migraine is also associated with sympathetic insufficiency. This study investigates the effects of VIP on the number of mast cells in the dura mater and on c-Fos expression in the trigeminal nucleus of sympathectomized rats. Experiments were carried out with 32 Sprague-Dawley male rats with body weights of 200-250 g. In the sympathectomized group, the left superior cervical sympathetic ganglion was removed. In the sympathectomized + VIP group, postoperative VIP 25 ng/kg/day (0.2 ml) was administered for 5 days. In the sham group, the ganglion and nerves were exposed but not dissected. Dura maters were stained with toluidine blue, and brainstems were labeled by indirect immunohistochemistry for c-Fos. Sympathectomy significantly increased the number of mast cells in both the ipsilateral and the contralateral dura mater (P < 0.001). VIP decreased the number of mast cells in both sides of the dura mater in sympathectomized rats. VIP also decreased c-Fos expression in the ipsilateral trigeminal nucleus of sympathectomized rats (P < 0.001). In the context of an experimental superior cervical ganglionectomy model of migraine, VIP is an efficient modulator of neurogenic inflammation of the dura., (© 2014 Wiley Periodicals, Inc.)

Published

2015

28. Biaxial response of ovine spinal cord dura mater.

Author

Shetye SS, Deault MM, and Puttlitz CM

Subjects

Animals, Anisotropy, Biomechanical Phenomena, Stress, Mechanical, Weight-Bearing, Dura Mater cytology, Dura Mater physiology, Materials Testing, Mechanical Phenomena, Sheep, Spinal Cord

Abstract

The dura mater performs a major functional role in the stability and mechanical response of the spinal cord complex. Computational techniques investigating the etiology of spinal cord injury require an accurate mechanical description of the dura mater. Previous studies investigating the mechanical response of the dura mater have reported conflicting results regarding the anisotropic stiffness of the dura in the longitudinal and circumferential direction. The aim of this study was to investigate the biaxial response of the dura mater in order to establish the tissue level mechanical behavior under physiological loading scenarios. To this end, square sections of the dura were tested in a custom biaxial setup under a comprehensive uniaxial and biaxial loading protocol. The resultant data were fit via a transversely isotropic continuum model and an anisotropic continuum constitutive model. The transversely isotropic formulation failed to accurately predict the dura mater׳s uniaxial behavior. The anisotropic formulation accurately predicted the uniaxial response in both longitudinal and circumferential directions. Significantly higher stiffness (p<0.0001) was observed in the circumferential direction as compared to the longitudinal direction. Further, the longitudinal direction displayed a significantly lower degree of nonlinearity (p<0.045) and significantly higher degree of collagen fiber dispersion (p<0.032) as compared to the circumferential direction. Results indicate that the dura mater has differential mechanical response in the longitudinal and circumferential directions and future studies should utilize an anisotropic two fiber family continuum model to accurately describe dura mater mechanics., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published

2014

29. Mast cells in the human dura: effects of age and dural bleeding--authors' reply.

Author

Varatharaj A, Squier W, and Mack J

Subjects

Humans, Cellular Senescence, Dura Mater cytology, Hematoma, Subdural pathology, Mast Cells

Published

2013

30. Mast cells in the human dura: effects of age and dural bleeding.

Author

Greeley CS and Karst WA

Subjects

Humans, Cellular Senescence, Dura Mater cytology, Hematoma, Subdural pathology, Mast Cells

Published

2013

31. Is there an identifiable intact medial wall of the cavernous sinus? Macro- and microscopic anatomical study using sheet plastination.

Author

Diao Y, Liang L, Yu C, and Zhang M

Subjects

Aged, Aged, 80 and over, Cavernous Sinus anatomy & histology, Cavernous Sinus cytology, Dura Mater anatomy & histology, Dura Mater cytology, Female, Humans, Male, Meninges anatomy & histology, Meninges cytology, Middle Aged, Pia Mater anatomy & histology, Pia Mater cytology, Pituitary Gland surgery, Pituitary Neoplasms diagnosis, Pituitary Neoplasms surgery, Cavernous Sinus pathology, Dura Mater pathology, Meninges pathology, Pia Mater pathology, Pituitary Gland pathology

Abstract

Background: The medial wall of the cavernous sinus is believed to play a significant role in determining the direction of growth of pituitary adenomas and in planning pituitary surgery. However, it remains unclear whether there is a dural wall between the pituitary gland and the cavernous sinus., Objective: To identify and trace the membranelike structures medial to the cavernous sinus and around the pituitary gland and their relationships with surrounding structures., Methods: Sixteen cadavers (7 females and 9 males; age range, 54-89 years; mean age, 77 years) were used in this study and prepared as 16 sets of transverse (5 sets), coronal (2 sets), and sagittal (9 sets) plastinated sections that were examined at both macro- and microscopic levels., Results: The pituitary gland was fully enclosed in a fibrous capsule, but the components and thickness of the capsule varied on different aspects of the gland. The meningeal dural layer was sandwiched between the anterosuperior aspect of the gland capsule and the cavernous sinus. Posteroinferiorly, however, this dural layer disappeared as it fused with the capsule. A weblike loose fibrous network connected the capsule, carotid artery, venous plexus, and the dura of the middle cranial fossa., Conclusion: The medial wall of the cavernous sinus consists of both the meningeal dura and weblike loose fibrous network, which are located at the anterosuperior and posteroinferior aspects, respectively.

Published

2013

32. Biological effects of cobalt-chromium nanoparticles and ions on dural fibroblasts and dural epithelial cells.

Author

Behl B, Papageorgiou I, Brown C, Hall R, Tipper JL, Fisher J, and Ingham E

Subjects

Animals, Cell Survival drug effects, Cells, Cultured, Epithelial Cells cytology, Fibroblasts cytology, Interleukin-6 metabolism, Interleukin-8 metabolism, Swine, Chromium chemistry, Cobalt chemistry, Dura Mater cytology, Epithelial Cells drug effects, Epithelial Cells metabolism, Fibroblasts drug effects, Fibroblasts metabolism, Nanoparticles adverse effects, Nanoparticles chemistry

Abstract

The introduction of metal-on-metal total disc replacements motivated studies to evaluate the effects of cobalt-chromium (CoCr) nanoparticles on cells of the dura mater. Porcine fibroblasts and epithelial cells isolated from the dura mater were cultured with clinically-relevant CoCr nanoparticles and the ions, generated by the particles over 24 h, at doses up to 121 μm(3)per cell. Cell viability and production of proinflammatory cytokines was assessed over 4 days. The capacity of the particles to induce oxidative stress in the cells was evaluated at 24 h. The CoCr particles and their ions significantly reduced the viability of the dural epithelial cells in a dose-dependent manner but not the fibroblasts. Both cell types secreted IL-8 in response to particle exposure at doses of 60.5 μm(3) (epithelial cells) and 121 μm(3) (fibroblasts, epithelial cells) per cell. No significant release of IL-6 was observed in both cell types at any dose. Reactive oxygen species were induced in both cell types at 50 μm(3) per cell after 24 h exposure. The data suggested novel differences in the resistance of the dural epithelial cells and fibroblasts to CoCr nanoparticle/ion toxicity and demonstrated the inflammatory potential of the particles. The data contributes to a greater understanding of the potential biological consequences of the use of metal-on-metal total disc prostheses., (Copyright © 2013 Elsevier Ltd. All rights reserved.)

Published

2013

33. A new model for dura mater healing: human dural fibroblast culture.

Author

Goldschmidt E, Hem S, Ajler P, Ielpi M, Loresi M, Giunta D, Carrizo A, Yampolsky C, and Argibay P

Subjects

Anti-Inflammatory Agents pharmacology, Cell Proliferation drug effects, Cellulose, Oxidized pharmacology, Dexamethasone pharmacology, Dura Mater drug effects, Fibrin Foam pharmacology, Fibroblasts drug effects, Hemostatics pharmacology, Humans, Immunohistochemistry, Cell Culture Techniques methods, Dura Mater cytology, Fibroblasts cytology, Models, Biological, Wound Healing drug effects

Abstract

Objective: Dura mater healing is crucial to prevent cerebrospinal fluid (CSF) leaks after neurosurgical procedures. Biological mechanisms leading to dural closure are only partially understood and have been studied in animals exclusively. We studied an in vitro model of dural closure which uses human cells., Materials and Methods: We used human dura intended for disposal after surgery. Explant primary cultures were performed. Cells were characterized through common staining and immunohistochemistry. A cell growth curve was elaborated and the effect of dexamethasone on cell count was assessed. Spongostan®, oxidized regenerated cellulose and autologous plastic materials were also evaluated for their effect on cellular growth., Results: All specimens showed growth in fusiform cells, which project pseudopods and fuse into spindles. Cells showed desmin and vimentin positivity, and were negative for all the other stains, behaving phenotypically like fibroblasts. No collagen base was necessary for cell growth. Dexamethasone decreased cell count in the primary culture as well as in the explant, and reduced the cell proliferation marker Ki-67. Spongostan® was successfully used as a graft, and fibroblast cultures were additionally developed with muscle, pericranium, galea, and fascia. Oxidized cellulose induced cell death by lowering the pH of the solution., Discussion: According to the findings, unlike mini-pigs and rabbits, in humans, dural fibroblast sensitivity to collagen seems to be lower. Dexamethasone inhibits fibroblast invasion, which is the biological base of wound dehiscence in cranial surgery. Although Spongostan is useful, Surgicel® can lower the media pH, thereby inhibiting cellular growth.

Published

2013

34. Comparison between two surgical techniques for prenatal correction of meningomyelocele in sheep.

Author

Herrera SR, Leme RJ, Valente PR, Caldini EG, Saldiva PH, and Pedreira DA

Subjects

Animals, Disease Models, Animal, Dura Mater cytology, Dura Mater surgery, Female, Inventions, Obstetric Labor, Premature, Pregnancy, Sheep, Fetal Therapies, Fetoscopy methods, Fetus surgery, Meningomyelocele surgery, Neurosurgical Procedures methods

Abstract

Objective: To compare the classical neurosurgical technique with a new simplified technique for prenatal repair of a myelomeningocele-like defect in sheep., Methods: A myelomeningocele-like defect (laminectomy and dural excision) was created in the lumbar region on day 90 of gestation in 9 pregnant sheep. Correction technique was randomized. In Group 1 the defect was corrected using the classic neurosurgical technique of three-layer suture (dura mater, muscle and skin closure) performed by a neurosurgeon. In Group 2, a fetal medicine specialist used a biosynthetic cellulose patch to protect the spinal cord and only the skin was sutured above it. Near term (day 132 of gestation) fetuses were sacrificed for pathological analysis., Results: There were two miscarriages and one maternal death. In total, six cases were available for pathological analysis, three in each group. In Group 1, there were adherence of the spinal cord to the scar (meningo-neural adhesion) and spinal cord architecture loss with posterior funiculus destruction and no visualization of grey matter. In Group 2, we observed in all cases formation of a neo-dura mater, separating the nervous tissue from adjacent muscles, and preserving the posterior funiculus and grey matter., Conclusion: The new simplified technique was better than the classic neurosurgical technique. It preserved the nervous tissue and prevented the adherence of the spinal cord to the scar. This suggests the current technique used for the correction of spina bifida in humans may need to be reassessed.

Published

2012

35. Precise control of osteogenesis for craniofacial defect repair: the role of direct osteoprogenitor contact in BMP-2-based bioprinting.

Author

Smith DM, Cray JJ Jr, Weiss LE, Dai Fei EK, Shakir S, Rottgers SA, Losee JE, Campbell PG, and Cooper GM

Subjects

Acellular Dermis, Animals, Craniotomy, Dura Mater cytology, Male, Mice, Mice, Inbred C57BL, Parietal Bone surgery, Stem Cells, Bioprinting methods, Bone Morphogenetic Protein 2 administration & dosage, Bone Regeneration physiology, Guided Tissue Regeneration methods, Parietal Bone physiology

Abstract

Background: Success with bone morphogenetic protein-2 (BMP-2) has been widely reported in the osseous reconstruction of large calvarial defects. These efforts have required enormous doses of BMP-2 and are not sufficiently refined to facilitate the detail-oriented repair required for intricate craniofacial structures. We have previously shown that inkjet-based bioprinting technologies allow for precisely customized low-dose protein patterns to induce spatially regulated osteogenesis. Here, we investigate the importance of direct contact between bioprinted BMP-2 and the dura mater (a source of osteoprogenitors) in mediating calvarial healing., Methods: Five-millimeter osseous defects were trephinated in mouse parietal bones (N=8). Circular acellular dermal matrix (ADM) implants were prepared such that 1 semicircle of 1 face per implant was printed with BMP-2 bio-ink. These implants were then placed ink-toward (N=3) or ink-away (N=5) from the underlying dura mater. After 4 weeks, osteogenesis was assessed in each of the 4 possible positions (BMP-2-printed area toward dura, BMP-2-printed area away from dura, unprinted area toward dura, and unprinted area away from dura) by faxitron., Results: The BMP-2-printed portion of the ADM generated bone covering an average of 66.5% of its surface area when it was face-down (printed surface directly abutting dura mater). By comparison, the BMP-2-printed portion of the ADM generated bone covering an average of only 21.3% of its surface area when it was face-up (printed surface away from dura). Similarly, the unprinted portion of the ADM generated an average of only 18.6% osseous coverage when face-down and 18.4% when face-up., Conclusions: We have previously shown that inkjet-based bioprinting has the potential to significantly enhance the role of regenerative therapies in craniofacial surgery. This technology affords the precise control of osteogenesis necessary to reconstruct this region's intricate anatomical architecture. In the present study, we demonstrate that direct apposition of BMP-2-printed ADM to a source of osteoprogenitor cells (in this case dura mater) is necessary for bio-ink-directed osteogenesis to occur. These results have important implications for the design of more complex bioprinted osseous structures.

Published

2012

36. Expression of the transient receptor potential channels TRPV1, TRPA1 and TRPM8 in mouse trigeminal primary afferent neurons innervating the dura.

Author

Huang D, Li S, Dhaka A, Story GM, and Cao YQ

Subjects

Animals, Calcitonin Gene-Related Peptide metabolism, Cell Size, Dura Mater cytology, Face innervation, Mice, Mice, Inbred C57BL, Plant Lectins metabolism, Skin innervation, TRPA1 Cation Channel, Dura Mater metabolism, Neurons, Afferent cytology, Neurons, Afferent metabolism, TRPM Cation Channels metabolism, TRPV Cation Channels metabolism, Transient Receptor Potential Channels metabolism, Trigeminal Ganglion cytology

Abstract

Background: Migraine and other headache disorders affect a large percentage of the population and cause debilitating pain. Activation and sensitization of the trigeminal primary afferent neurons innervating the dura and cerebral vessels is a crucial step in the "headache circuit". Many dural afferent neurons respond to algesic and inflammatory agents. Given the clear role of the transient receptor potential (TRP) family of channels in both sensing chemical stimulants and mediating inflammatory pain, we investigated the expression of TRP channels in dural afferent neurons., Methods: We used two fluorescent tracers to retrogradely label dural afferent neurons in adult mice and quantified the abundance of peptidergic and non-peptidergic neuron populations using calcitonin gene-related peptide immunoreactivity (CGRP-ir) and isolectin B4 (IB4) binding as markers, respectively. Using immunohistochemistry, we compared the expression of TRPV1 and TRPA1 channels in dural afferent neurons with the expression in total trigeminal ganglion (TG) neurons. To examine the distribution of TRPM8 channels, we labeled dural afferent neurons in mice expressing farnesylated enhanced green fluorescent protein (EGFPf) from a TRPM8 locus. We used nearest-neighbor measurement to predict the spatial association between dural afferent neurons and neurons expressing TRPA1 or TRPM8 channels in the TG., Results and Conclusions: We report that the size of dural afferent neurons is significantly larger than that of total TG neurons and facial skin afferents. Approximately 40% of dural afferent neurons exhibit IB4 binding. Surprisingly, the percentage of dural afferent neurons containing CGRP-ir is significantly lower than those of total TG neurons and facial skin afferents. Both TRPV1 and TRPA1 channels are expressed in dural afferent neurons. Furthermore, nearest-neighbor measurement indicates that TRPA1-expressing neurons are clustered around a subset of dural afferent neurons. Interestingly, TRPM8-expressing neurons are virtually absent in the dural afferent population, nor do these neurons cluster around dural afferent neurons. Taken together, our results suggest that TRPV1 and TRPA1 but not TRPM8 channels likely contribute to the excitation of dural afferent neurons and the subsequent activation of the headache circuit. These results provide an anatomical basis for understanding further the functional significance of TRP channels in headache pathophysiology.

Published

2012

37. Influence of sex, estrous cycle, and estrogen on intracranial dural mast cells.

Author

Boes T and Levy D

Subjects

Animals, Brain metabolism, Dura Mater metabolism, Female, Male, Migraine Disorders metabolism, Migraine Disorders pathology, Ovariectomy, Rats, Rats, Sprague-Dawley, Spleen cytology, Brain cytology, Dura Mater cytology, Estrogens physiology, Estrous Cycle physiology, Mast Cells cytology, Sex Characteristics

Abstract

Background: The frequency of migraine headaches is higher in women than in men and in susceptible women attacks are related to changes in ovarian hormone levels. Intracranial mast cells (MCs) are likely to have a role in migraine headache genesis, and changes in the dural MC population might influence headache susceptibility. The present study thus tested the hypothesis that sex and ovarian hormones influence the density and phenotypic makeup of dural MCs., Methods: Histochemistry combined with quantitative analyses was used to investigate sex differences, estrous cycle and ovarian hormones on dural MC density, phenotype and degranulation level in male and female rats., Results: Our data show that in female rats, dural MC density fluctuates during the estrous cycle and is overall higher than in males. In ovariectomized rats, estradiol, but not progesterone, promoted an increase in dural MC density. This effect was abolished by a splenectomy, suggesting estrogen-related recruitment of MCs from the spleen. Finally, our data suggest that the phenotypic make up of dural MCs, which represents the level of cellular maturity, is also governed by changes in estrogen levels., Conclusions: Given the potential role of dural MCs in triggering headache, our data suggest that estrogen-related modulation of dural MC density and phenotypic makeup could have a role in mediating the higher frequency and severity of headaches such as migraine, in women.

Published

2012

38. Tissue interactions between craniosynostotic dura mater and bone.

Author

Cooper GM, Durham EL, Cray JJ Jr, Siegel MI, Losee JE, and Mooney MP

Subjects

Alkaline Phosphatase metabolism, Analysis of Variance, Animals, Cell Differentiation, Cell Proliferation, Coculture Techniques, Cranial Sutures metabolism, Cranial Sutures surgery, Craniosynostoses metabolism, Dura Mater metabolism, Osteogenesis physiology, Phenotype, Polytetrafluoroethylene, Rabbits, Bone Morphogenetic Protein 4 pharmacology, Cranial Sutures cytology, Craniosynostoses surgery, Dura Mater cytology

Abstract

Background: Cells within the dura mater have been implicated in the determination of suture patency and fusion. Craniosynostosis (CS), the premature fusion of 1 or more of the cranial sutures, could result from abnormal control over the differentiation of osteoprogenitor cells from the dura mater. This study tested whether dura mater cells derived from rabbits with congenital CS were different from cells derived from normal rabbits and investigated the effects that CS dura mater had on osteogenic differentiation in vitro and in vivo., Methods: Cells were derived from the dura mater from wild-type rabbits (WT; n = 23) or CS rabbits (n = 16). Cells were stimulated with bone morphogenetic protein 4, and alkaline phosphatase (ALP) expression and cell proliferation were assessed. Dura mater-derived cells were also cocultured with primary rabbit bone-derived cells, and ALP was assessed. Finally, interactions between the dura mater and overlying tissues were manipulated in vivo., Results: Craniosynostotic dura mater-derived cells proliferated faster than did WT cells but were not more ALP positive. Coculture experiments showed that CS dura mater cells induced increased ALP activity in CS bone-derived cells, but not in WT bone-derived cells. In vivo experiments showed that a physical barrier successfully inhibited dura mater-derived osteogenesis., Conclusions: Coculture of CS bone- and CS dura mater-derived cells evoked an abnormal phenotype in vitro. Covering the CS dura mater led to decreased bone formation in vivo. Further investigations will focus on the signaling molecules involved in the communication between these 2 CS tissue types in vitro and in vivo.

Published

2012

39. Mast cells in the human dura: effects of age and dural bleeding.

Author

Varatharaj A, Mack J, Davidson JR, Gutnikov A, and Squier W

Subjects

Adult, Aged, Cell Count methods, Child, Child, Preschool, Dura Mater pathology, Dura Mater physiopathology, Fetus, Hematoma, Subdural physiopathology, Humans, Infant, Infant, Newborn, Middle Aged, Young Adult, Cellular Senescence physiology, Dura Mater cytology, Hematoma, Subdural pathology, Mast Cells physiology

Abstract

Background: Animal studies have shown that the dura mater contains mast cells. We investigated the density of mast cells in the human dura mater, and the changes associated with subdural haemorrhage (SDH)., Methods: Samples of the human dura were stained with tryptase antibody and were examined for mast cells. We used control cases with no dural bleeding (n = 9) and cases of fresh (n = 24) and old (n = 18) dural haemorrhage., Results: Mast cells were easily found in dural samples. The mean density in controls (11.05 cells per mm(2)) was less than that in fresh SDH (15.69), which was less than that in old SDH (23.09)., Conclusions: Subdural haemorrhage is associated with an increase in dural mast cell density, and the density increases as the haematoma ages. We hypothesise that dural mast cells may contribute to neurogenic inflammation and the clinical features of subdural haemorrhage.

Published

2012

40. K(ATP) channel openers in the trigeminovascular system.

Author

Ploug KB, Amrutkar DV, Baun M, Ramachandran R, Iversen A, Lund TM, Gupta S, Hay-Schmidt A, Olesen J, and Jansen-Olesen I

Subjects

ATP-Binding Cassette Transporters metabolism, Animals, Calcitonin Gene-Related Peptide metabolism, Cell Degranulation drug effects, Cell Degranulation physiology, Cromakalim pharmacology, Diazoxide pharmacology, Disease Models, Animal, Dura Mater blood supply, Dura Mater cytology, KATP Channels metabolism, Male, Mast Cells drug effects, Mast Cells metabolism, Migraine Disorders chemically induced, Potassium Channels, Inwardly Rectifying metabolism, Rats, Rats, Sprague-Dawley, Receptors, Drug metabolism, Sulfonylurea Receptors, Trigeminal Caudal Nucleus blood supply, Trigeminal Caudal Nucleus drug effects, Trigeminal Ganglion blood supply, Trigeminal Ganglion drug effects, Vasodilator Agents pharmacology, ATP-Binding Cassette Transporters genetics, KATP Channels genetics, Migraine Disorders physiopathology, Potassium Channels, Inwardly Rectifying genetics, Receptors, Drug genetics, Trigeminal Caudal Nucleus physiology, Trigeminal Ganglion physiology

Abstract

Background: The ATP-sensitive K(+) (K(ATP)) channel openers levcromakalim and pinacidil are vasodilators that induce headache in healthy people. The neuropeptide calcitonin gene-related peptide (CGRP) induces headache in healthy people and migraine in migraineurs, potentially through a mechanism that involves opening of vascular or neuronal K(ATP) channels and mast cell degranulation. Using rat as a model, we studied the molecular presence of K(ATP) channels in the trigeminovascular system. Furthermore, we examined whether K(ATP) channel openers stimulate the in vitro release of CGRP and whether they degranulate dural mast cells., Methods: mRNA and protein expression of K(ATP) channel subunits were studied in the trigeminal ganglion (TG) and trigeminal nucleus caudalis (TNC) by qPCR and western blotting. In vitro CGRP release was studied after application of levcromakalim (1 µM) and diazoxide (10 µM) to freshly isolated rat dura mater, TG and TNC. Rat dural mast cells were challenged in situ with levcromakalim (10(-5) M) to study its potential degranulation effect., Results: mRNA and protein of K(ATP) channel subunits Kir6.1, Kir6.2, SUR1 and SUR2B were identified in the TG and TNC. K(ATP) channel openers did not release or inhibit capsaicin-induced CGRP release from dura mater, TG or TNC. They did also not induce dural mast cell degranulation., Conclusions: K(ATP) channel openers do not interact with CGRP release or mast cell degranulation. Activation of these channels in the CNS is antinociceptive and therefore cannot explain the headache induced by K(ATP) channel openers. Thus, they are likely to induce headache by interaction with extracerebral K(ATP) channels, probably the SUR2B isoforms.

Published

2012

41. Use of postmortem human dura mater and scalp for deriving human fibroblast cultures.

Author

Bliss LA, Sams MR, Deep-Soboslay A, Ren-Patterson R, Jaffe AE, Chenoweth JG, Jaishankar A, Kleinman JE, and Hyde TM

Subjects

Adult, Body Mass Index, Cell Differentiation, Cell Proliferation, Female, Humans, Male, Middle Aged, Specimen Handling, Time Factors, Autopsy methods, Cell Culture Techniques, Dura Mater cytology, Fibroblasts cytology, Induced Pluripotent Stem Cells cytology, Scalp cytology

Abstract

Fibroblasts can be collected from deceased individuals, grown in culture, reprogrammed into induced pluripotent stem cells (iPSCs), and then differentiated into a multitude of cell types, including neurons. Past studies have generated iPSCs from somatic cell biopsies from either animal or human subjects. Previously, fibroblasts have only been successfully cultured from postmortem human skin in two studies. Here we present data on fibroblast cell cultures generated from 146 scalp and/or 53 dura mater samples from 146 postmortem human brain donors. In our overall sample, the odds of successful dural culture was almost two-fold compared with scalp (OR = 1.95, 95% CI: [1.01, 3.9], p = 0.047). Using a paired design within subjects for whom both tissues were available for culture (n = 53), the odds of success for culture in dura was 16-fold as compared to scalp (OR = 16.0, 95% CI: [2.1-120.6], p = 0.0007). Unattended death, tissue donation source, longer postmortem interval (PMI), and higher body mass index (BMI) were associated with unsuccessful culture in scalp (all p<0.05), but not in dura. While scalp cells proliferated more and grew more rapidly than dura cells [F (1, 46) = 12.94, p<0.008], both tissues could be generated and maintained as fibroblast cell lines. Using a random sample of four cases, we found that both postmortem scalp and dura could be successfully reprogrammed into iPSC lines. Our study demonstrates that postmortem dura mater, and to a lesser extent, scalp, are viable sources of living fibroblasts for culture that can be used to generate iPSCs. These tissues may be accessible through existing brain tissue collections, which is critical for studying disorders such as neuropsychiatric diseases.

Published

2012

42. Tumor necrosis factor-α induces sensitization of meningeal nociceptors mediated via local COX and p38 MAP kinase actions.

Author

Zhang XC, Kainz V, Burstein R, and Levy D

Subjects

Action Potentials drug effects, Animals, Disease Models, Animal, Dura Mater cytology, Dura Mater metabolism, Endothelial Cells metabolism, Enzyme Inhibitors pharmacology, Imidazoles pharmacology, Male, Physical Stimulation adverse effects, Pyrazoles pharmacology, Pyridines pharmacology, Rats, Rats, Sprague-Dawley, Receptors, Tumor Necrosis Factor, Type I metabolism, Sensory Receptor Cells drug effects, Time Factors, Trigeminal Ganglion cytology, Cyclooxygenase 1 metabolism, Hyperalgesia chemically induced, Hyperalgesia metabolism, Membrane Proteins metabolism, Sensory Receptor Cells physiology, Tumor Necrosis Factor-alpha pharmacology, p38 Mitogen-Activated Protein Kinases metabolism

Abstract

The proinflammatory cytokine TNF-α has been shown to promote activation and sensitization of primary afferent nociceptors. The downstream signaling processes that play a role in promoting this neuronal response remain however controversial. Increased TNF-α plasma levels during migraine attacks suggest that local interaction between this cytokine and intracranial meningeal nociceptors plays a role in promoting the headache. Here, using in vivo single unit recording in the trigeminal ganglia of anesthetized rats, we show that meningeal TNF-α action promotes a delayed mechanical sensitization of meningeal nociceptors. Using immunohistochemistry, we provide evidence for non-neuronal localization of the TNF receptors TNFR1 to dural endothelial vascular cells and TNFR2 to dural resident macrophages as well as to some CGRP-expressing dural nerve fibers. We also demonstrate that meningeal vascular TNFR1 is co-localized with COX-1 while the perivascular TNFR2 is co-expressed with COX-2. We further report here for the first time that TNF-α evoked sensitization of meningeal nociceptors is dependent upon local action of cyclooxygenase (COX). Finally, we show that local application of TNF-α to the meninges evokes activation of the p38 MAP kinase in dural blood vessels that also express TNFR1 and that pharmacological blockade of p38 activation inhibits TNF-α evoked sensitization of meningeal nociceptors. Our study suggests that meningeal action of TNF-α could play an important role in the genesis of intracranial throbbing headaches such as migraine through a mechanism that involves at least part activation of non-neuronal TNFR1 and TNFR2 and downstream activation of meningeal non-neuronal COX and the p38 MAP kinase., (Copyright © 2010 International Association for the Study of Pain. Published by Elsevier B.V. All rights reserved.)

Published

2011

43. Use of a collagen biomatrix (TissuDura) for dura repair: a long-term neuroradiological and neuropathological evaluation.

Author

Parlato C, di Nuzzo G, Luongo M, Parlato RS, Accardo M, Cuccurullo L, and Moraci A

Subjects

Dura Mater chemistry, Dura Mater cytology, Follow-Up Studies, Humans, Time, Biocompatible Materials therapeutic use, Collagen chemistry, Collagen therapeutic use, Dura Mater surgery, Membranes, Artificial, Neurosurgical Procedures methods, Plastic Surgery Procedures methods

Abstract

Purpose: The aim of this study was to evaluate the clinical, neuroradiological, and neuropathological outcomes of patients treated with equine collagen foil (TissuDura) as a dura mater substitute during cranial and spinal neurosurgical procedures., Materials and Methods: All patients treated at the Department of Neurosurgery of the Second University of Naples with TissuDura between 2005 and 2009 were included. Dural reconstruction was performed using TissuDura, overlaid 1 cm over the dural defect with additional fixation using fibrin glue. No surgical sutures were used. Patients underwent postoperative contrast-enhanced magnetic resonance scans at 1 week, 1 month, and 1 year after surgery to detect any cerebrospinal fluid (CSF) leaks, infections, inflammations, or CSF circulation in the surgical region., Results: Dural reconstruction was performed in 74 patients, including 50 patients with tumors, two with C2 neurinoma, two with acoustic neurinoma, six with Chiari I malformation, two with severe head injury, and 12 requiring spinal surgery. Clinical and neuroradiological findings were normal and no signs of graft rejection or CSF leaks at postoperative follow-up were observed. In two cases of atypical meningioma, re-operation of the dural reconstruction was performed after 1 year. No adherences between brain and neodura were detected, and histopathological investigations demonstrated dural regeneration., Conclusions: Following dural reconstructions with TissuDura without surgical sutures, no local toxicity or complications were observed for up to 1 year. TissuDura demonstrated elasticity, non-reactivity, and good adaptability. The overlay technique using fibrin glue was simple and fast. Future studies and longer follow-up are needed to confirm the efficacy of TissuDura.

Published

2011

44. Radially aligned, electrospun nanofibers as dural substitutes for wound closure and tissue regeneration applications.

Author

Xie J, Macewan MR, Ray WZ, Liu W, Siewe DY, and Xia Y

Subjects

Animals, Dura Mater drug effects, Fibroblasts cytology, Fibroblasts drug effects, Microscopy, Fluorescence, Polyesters chemistry, Polyesters pharmacology, Rabbits, Dura Mater cytology, Electricity, Guided Tissue Regeneration methods, Nanofibers chemistry, Nanomedicine methods, Tissue Scaffolds chemistry, Wound Healing

Abstract

This paper reports the fabrication of scaffolds consisting of radially aligned poly(ε-caprolactone) nanofibers by utilizing a collector composed of a central point electrode and a peripheral ring electrode. This novel class of scaffolds was able to present nanoscale topographic cues to cultured cells, directing and enhancing their migration from the periphery to the center. We also established that such scaffolds could induce faster cellular migration and population than nonwoven mats consisting of random nanofibers. Dural fibroblast cells cultured on these two types of scaffolds were found to express type I collagen, the main extracellular matrix component in dural mater. The type I collagen exhibited a high degree of organization on the scaffolds of radially aligned fibers and a haphazard distribution on the scaffolds of random fibers. Taken together, the scaffolds based on radially aligned, electrospun nanofibers show great potential as artificial dural substitutes and may be particularly useful as biomedical patches or grafts to induce wound closure and/or tissue regeneration.

Published

2010

45. Dura in the pathogenesis of syndromic craniosynostosis: fibroblast growth factor receptor 2 mutations in dural cells promote osteogenic proliferation and differentiation of osteoblasts.

Author

Ang BU, Spivak RM, Nah HD, and Kirschner RE

Subjects

Acrocephalosyndactylia genetics, Adenoviridae genetics, Alkaline Phosphatase analysis, Animals, Arginine genetics, Biomarkers analysis, Cell Differentiation physiology, Cell Proliferation, Cells, Cultured, Coculture Techniques, Coloring Agents, Core Binding Factor Alpha 1 Subunit genetics, Craniofacial Dysostosis genetics, Cysteine genetics, Dura Mater physiology, Genetic Vectors genetics, Mice, Osteogenesis genetics, Osteopontin genetics, Phenylalanine genetics, Syndrome, Tetrazolium Salts, Thiazoles, Craniosynostoses etiology, Dura Mater cytology, Osteoblasts physiology, Osteogenesis physiology, Point Mutation genetics, Receptor, Fibroblast Growth Factor, Type 2 genetics

Abstract

Mutations in fibroblast growth factor receptor 2 (FGFR2), a transmembrane receptor expressed in suture mesenchyme, osteogenic fronts, and dura, have been implicated in the etiopathogenesis of craniosynostosis syndromes. The C278F- and P253R-FGFR2 mutations result in Crouzon and Apert syndromes, respectively. The dura mater plays a critical role in the formation and maintenance of cranial sutures. However, its role in syndromic craniosynostosis remains unclear. This study examines the influence of FGFR2 mutations in dural cells on osteoblast proliferation and differentiation. Primary cultures of dural cells and osteoblasts were established, and adenoviral-FGFR2 constructs were prepared by subcloning mutant (C278F and P253R) FGFR2 constructs into adenovirus. Dural cells were infected with adenovirus, and dural protein expression was confirmed by immunostaining. Infected dural cells were cocultured with osteoblasts using a transwell system for 7 days. Dural cells infected with null adenovirus served as the negative control. In separate cultures, osteoblasts were directly infected with the adenoviral-FGFR2 constructs. Osteoblast proliferation was analyzed by 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide (MTT) assay, and differentiation was analyzed by alkaline phosphatase assay, histochemical staining, and gene expression studies. Osteoblasts directly infected with the Crouzon (C278F-FGFR2) mutation demonstrated an increase in cell proliferation (P < 0.05). Osteoblasts directly infected with the Apert (P253R-FGFR2) mutation demonstrated an increase in alkaline phosphatase activity. In coculture experiments, osteoblasts cocultured with Crouzon-transformed dural cells demonstrated increased cell proliferation (P < 0.05), whereas osteoblasts cocultured with Apert-transformed dural cells showed an increase in alkaline phosphatase activity (P < 0.05). In addition, osteogenic gene expression (alkaline phosphatase, osteopontin, and runx2) were up-regulated in osteoblasts cocultured with Apert-expressing dural cells. These experiments suggest that FGFR2 mutations in dural cells alter normal dural signaling. Apert mutations promote osteodifferentiation, whereas Crouzon mutations result in enhanced cell proliferation. These mutations may induce craniosynostosis in part through the influence of mutation-induced constitutive signaling in the dura, with subsequent enhancement of dural-mediated osteogenesis.

Published

2010

46. Expression of extracellular matrix-proteins in perisellar connective tissue and dura mater.

Author

Knappe UJ, Fink T, Fisseler-Eckhoff A, and Schoenmayr R

Subjects

Aged, Aged, 80 and over, Biomarkers, Tumor analysis, Biomarkers, Tumor metabolism, Cavernous Sinus cytology, Collagen analysis, Collagen metabolism, Connective Tissue Cells cytology, Cranial Fossa, Middle cytology, Dura Mater cytology, Elastin analysis, Elastin metabolism, Extracellular Matrix Proteins analysis, Female, Fibronectins analysis, Fibronectins metabolism, Humans, Immunohistochemistry, Laminin analysis, Laminin metabolism, Male, Middle Aged, Neoplasm Invasiveness pathology, Neoplasm Invasiveness physiopathology, Pituitary Neoplasms metabolism, Pituitary Neoplasms pathology, Pituitary Neoplasms physiopathology, Sella Turcica cytology, Tenascin analysis, Tenascin metabolism, Vitronectin analysis, Vitronectin metabolism, Cavernous Sinus metabolism, Connective Tissue Cells metabolism, Cranial Fossa, Middle metabolism, Dura Mater metabolism, Extracellular Matrix Proteins metabolism, Sella Turcica metabolism

Abstract

Purpose: To describe the pattern of expression of extracellular matrix (ECM) proteins in perisellar connective tissue., Methods: Dural and perisellar specimens from ten individuals were investigated immunohistochemically for collagens I to IV, tenascin, fibronectin, elastin, laminin, and vitronectin., Findings: Collagen I and III and fibronectin were strongly expressed and collagen IV, tenascin, and vitronectin were moderately expressed in the boundaries of the sella and around the CS. In six of nine specimens from the anterior boundary of the sella, and in 11 of 19 samples from the lateral boundary of the sella (medial wall of CS), two different layers could be detected by the expression of different ECM proteins. None of the antigens generally allowed differentiation between two layers of the pituitary envelope., Conclusions: The pituitary boundary may consist of a single or a double layer, infrequently differentiated from each other by the expression of different ECM proteins.

Published

2010

47. Comparison of porcine acellular dermis and dura mater as natural scaffolds for bioengineering tympanic membranes.

Author

Deng Z, Wu J, Qiu J, Wang J, Tian Y, Li Y, and Jin Y

Subjects

Animals, Audiometry, Pure-Tone, Auditory Threshold drug effects, Biocompatible Materials pharmacology, Cells, Cultured, Dermis cytology, Dermis drug effects, Disease Models, Animal, Dura Mater cytology, Dura Mater drug effects, Fibroblasts cytology, Fibroblasts drug effects, Fibroblasts transplantation, Guinea Pigs, Sus scrofa, Tissue Culture Techniques, Tympanic Membrane transplantation, Tympanic Membrane Perforation pathology, Tympanic Membrane Perforation therapy, Wound Healing drug effects, Bioengineering methods, Dermis transplantation, Dura Mater transplantation, Tissue Scaffolds chemistry, Tympanic Membrane pathology

Abstract

Tympanic membrane (TM) perforation is a frequent cause of conductive hearing loss. The most popular surgical repair is autografting with temporalis fascia, although some disadvantages have been found with this method. Whether xenogeneous grafts produced by a tissue engineering approach could be used is unclear. The purpose of this study was to evaluate the possibility of bioengineering TM using porcine acellular dermis and dura mater with TM fibroblasts and to compare the effects of these two natural scaffolds. Both of the materials were prepared by sequentially using Triton X-100, nuclease solution, and freeze-drying technique. Histologically, both had porous structures without any cellular components. After seeding with TM fibroblasts isolated from guinea pigs, it was found that both of the materials could be used as scaffolds for bioengineering TM in vitro. In the in vivo study, chronic TM perforation models were successfully established in guinea pigs. From gross and histological examinations, most of TM perforations were healed after grafting these two bioengineered TMs using an underlay technique. Furthermore, auditory brainstem response audiometry was applied to determine the auditory threshold in each group. Results showed that hearing in the dura mater group seemed to undergo faster recovery in the early stage but in the end, no differences were found between the two groups. Two kinds of materials without cell seeding were used as controls. Porcine acellular dermis and dura mater are suitable scaffolds for bioengineering TMs.

Published

2009

48. Discussion. TGF-beta1 RNA interference in mouse primary dura cell culture: downstream effects on TGF receptors, FGF-2, and FGF-R1 mRNA levels.

Author

Ko SH, Behr B, and Longaker MT

Subjects

Animals, Cell Culture Techniques, Cranial Sutures metabolism, Craniosynostoses metabolism, Down-Regulation, Drug Delivery Systems, Dura Mater cytology, Mice, Mice, Inbred Strains, RNA, Messenger metabolism, RNA, Small Interfering pharmacology, Transfection, Transforming Growth Factor beta metabolism, Craniosynostoses genetics, Dura Mater metabolism, Fibroblast Growth Factor 2 metabolism, RNA Interference, RNA, Small Interfering metabolism, Receptor, Fibroblast Growth Factor, Type 1 metabolism, Receptors, Transforming Growth Factor beta metabolism, Transforming Growth Factor beta genetics

Published

2009

49. TGF-beta1 RNA interference in mouse primary dura cell culture: downstream effects on TGF receptors, FGF-2, and FGF-R1 mRNA levels.

Author

Gosain AK, Machol JA 4th, Gliniak C, and Halligan NLN

Subjects

Animals, Cell Culture Techniques, Cranial Sutures metabolism, Craniosynostoses metabolism, Down-Regulation, Dura Mater cytology, Mice, Mice, Inbred Strains, RNA, Messenger metabolism, RNA, Small Interfering pharmacology, Transfection, Craniosynostoses genetics, Dura Mater metabolism, Fibroblast Growth Factor 2 metabolism, RNA Interference, RNA, Small Interfering metabolism, Receptor, Fibroblast Growth Factor, Type 1 metabolism, Receptors, Transforming Growth Factor beta metabolism, Transforming Growth Factor beta genetics

Abstract

Background: Transforming growth factor (TGF)-beta1 and fibroblast growth factor (FGF)-2 have both been shown to have significant roles in the regulation of murine calvarial suture fusion. Methods to decrease gene expression of these cytokines and their respective receptors have been established, but because of side effects, clinical applications are limited. In this study, the authors examined the effect of TGF-beta1-specific small interfering RNA (siRNA) on the messenger RNA (mRNA) expression of TGF-beta1, its TGF-betaR1 and TGF-betaR2 receptors, and FGF-2 and its R1 receptor in murine dura cells., Methods: A primary dura cell line was established from CD-1 mice. Transfection efficiency using Lipofectamine was determined using BLOCKiT. Dura cells were transfected with serial concentrations of TGF-beta1 siRNA to determine the optimal dose. In subsequent experiments, cells were transfected with 16 nM TGF-beta1 siRNA and harvested on posttransfection days 4, 7, 10, and 14 for RNA isolation and quantitative polymerase chain reaction., Results: Optimal inhibition of TGF-beta1 mRNA expression was achieved at 16 nM siRNA. On posttransfection day 4, TGF-beta1 mRNA levels were significantly decreased but returned to baseline by day 14. TGF-betaR1 mRNA expression remained unaffected by transfection throughout the time course. However, TGF-betaR2, FGF-2, and FGF-R1 demonstrated significant inhibition of mRNA expression on posttransfection day 4., Conclusions: These results indicate that TGF-beta1 siRNA has the potential to alter the murine dura cytokines responsible for suture fusion in vitro. Manipulating underlying cranial suture biology with siRNA technology may ultimately allow control over suture fusion. This intervention may ultimately function as an effective adjunct to surgical intervention for craniosynostosis.

Published

2009

50. Localization of COX-1 and COX-2 in the intracranial dura mater of the rat.

Author

Zhang XC, Kainz V, Jakubowski M, Burstein R, Strassman A, and Levy D

Subjects

Animals, Blood Vessels metabolism, Calcitonin Gene-Related Peptide metabolism, Dura Mater cytology, Ectodysplasins metabolism, Macrophages metabolism, Male, Nitric Oxide Synthase Type III metabolism, Pia Mater metabolism, Rats, Rats, Sprague-Dawley, Vimentin metabolism, Cyclooxygenase 1 metabolism, Cyclooxygenase 2 metabolism, Dura Mater metabolism, Membrane Proteins metabolism

Abstract

Primary headaches such as migraine can be aborted by systemic administration of non-steroidal anti-inflammatory drugs (NSAIDs), potentially through the non-selective inhibition of cyclooxygenase (COX) activity in the intracranial meninges. In this study we have used single and double labeling immunohistochemistry to examine the distribution of the COX-1 and COX-2 isoforms in the intracranial dura mater of the rat and identify cell types that express them. COX-1 immunoreactivity was found in medium and small dural blood vessels and was co-expressed with the endothelial cell markers vimentin and the endothelial isoform of nitric oxide synthase (ecNOS). COX-1 was also found to be present in most dural mast cells. COX-2 was mainly expressed in ED2-positive resident dural macrophages. Constitutive COX-2 expression was also found in some axonal profiles, many of which were co-labeled with the nociceptor peptide marker CGRP. The findings suggest that NSAIDs may abort headache, at least in part, by inhibiting either neuronal or non-neuronal COX activity in the dura mater.

Published

2009