Your search keyword '"Morrison EE"' showing total 7 results

1. Adenomatous polyposis coli localization is both cell type and cell context dependent.

Author

Langford KJ, Lee T, Askham JM, and Morrison EE

Subjects

Alternative Splicing, Animals, Cell Adhesion physiology, Cell Line, Epithelial Cells cytology, Fibroblasts cytology, Microtubules metabolism, Protein Isoforms, Rats, Spindle Apparatus metabolism, Adenomatous Polyposis Coli Protein metabolism, Epithelial Cells metabolism, Fibroblasts metabolism

Abstract

The adenomatous polyposis coli (APC) tumor suppressor protein is mutated in most colorectal carcinomas. In addition to its role in WNT signaling it is proposed to be involved in both cell migration and mitosis. Although a variety of studies have shown an APC localization along lateral membranes of adjacent epithelial cells the existence of a cortical APC localization in mammalian cells remains controversial. To address this we have used matched rat epithelial (NRK-52E) and fibroblast (NRK-49F) cell lines to investigate the localization of APC. Subconfluent cultures of NRK-52E and -49F cells displayed microtubule-associated APC populations by immunostaining. However, confluent NRK-52E, but not -49F monolayers, exhibited a cortical APC distribution. Cortical APC localized in close proximity to a number of cell junction proteins in a microtubule-independent manner while calcium switch experiments suggested that APC was recruited to the cortex only when junction assembly was complete. Confluent NRK-49F and -52E cells also showed contrasting APC localizations in response to monolayer wounding. Our data suggests APC cortical localization is a feature of confluent epithelioid cells and that the subcellular distribution of APC is therefore dependent upon both cell type and context., (Copyright 2006 Wiley-Liss, Inc.)

Published

2006

2. Intrinsic chemotherapy resistance to the tubulin-binding antimitotic agents in renal cell carcinoma.

Author

Ferguson RE, Jackson SM, Stanley AJ, Joyce AD, Harnden P, Morrison EE, Patel PM, Phillips RM, Selby PJ, and Banks RE

Subjects

ATP Binding Cassette Transporter, Subfamily B, Member 1 metabolism, Antineoplastic Agents, Phytogenic pharmacology, Blotting, Western, Cell Line, Cell Line, Tumor, Dose-Response Relationship, Drug, Down-Regulation, Humans, Immunohistochemistry, Inhibitory Concentration 50, Kidney drug effects, Membrane Transport Proteins metabolism, Multidrug Resistance-Associated Protein 2, Multidrug Resistance-Associated Proteins metabolism, Paclitaxel chemistry, Phenotype, Sensitivity and Specificity, Tetrazolium Salts pharmacology, Thiazoles pharmacology, Time Factors, Up-Regulation, Vinblastine pharmacology, Vincristine pharmacology, Antineoplastic Agents pharmacology, Carcinoma, Renal Cell drug therapy, Carcinoma, Renal Cell metabolism, Kidney Neoplasms drug therapy, Kidney Neoplasms metabolism, Tubulin chemistry

Abstract

Renal cancer is one of the most chemoresistant tumor types. Using a panel of 10 established renal cancer cell lines that have not been subjected to prior drug selection, the range of functional resistance phenotypes to the tubulin-binding agents paclitaxel, vinblastine, vincristine and patupilone (epothilone B, EPO906) was determined, together with expression of P-glycoprotein (PgP), multidrug resistance associated protein-2 (MRP2) and major vault protein (MVP) proteins. The IC(50) values for vincristine correlated positively with PgP expression (r = 0.73; p = 0.031), with values for paclitaxel and vinblastine just failing to reach significance. A significant positive correlation was observed for sensitivity to paclitaxel and MRP2 expression only (r = 0.8; p = 0.013). MVP expression did not correlate with sensitivity to any of the drugs examined. All cell lines exhibited much greater sensitivity to patupilone, demonstrating for the first time the potential use of patupilone in this cancer. In tissue samples from chemotherapy-naive renal cell carcinoma (RCC) patients, marked downregulation or absence of PgP in many tumor cells with expression levels more similar to sensitive cell lines rather than the resistant lines was seen. Similarly, MRP2 was absent or only weakly present in tumor cells, whereas MVP was very strongly upregulated in most tumor samples. This study illustrating discrepancies between results exclusively based on studies in cell lines and findings in vivo suggests that the role of PgP and MRP2 in intrinsic resistance in RCC in vivo may be less than expected from the in vitro findings and supports a potential role for MVP on the basis of in vivo expression studies., ((c) 2004 Wiley-Liss, Inc.)

Published

2005

3. Expression of neuron-specific markers by the vomeronasal neuroepithelium in six species of primates.

Author

Dennis JC, Smith TD, Bhatnagar KP, Bonar CJ, Burrows AM, and Morrison EE

Subjects

Aging physiology, Animals, Animals, Newborn, Biomarkers analysis, Biomarkers metabolism, Female, Immunohistochemistry, Male, Nerve Tissue Proteins analysis, Nerve Tissue Proteins biosynthesis, Olfactory Marker Protein, Olfactory Mucosa anatomy & histology, Olfactory Mucosa growth & development, Olfactory Receptor Neurons chemistry, Olfactory Receptor Neurons cytology, Phylogeny, Primates anatomy & histology, Species Specificity, Tubulin analysis, Ubiquitin Thiolesterase analysis, Ubiquitin Thiolesterase biosynthesis, Vomeronasal Organ anatomy & histology, Vomeronasal Organ growth & development, Olfactory Mucosa metabolism, Olfactory Receptor Neurons metabolism, Primates physiology, Vomeronasal Organ metabolism

Abstract

Vomeronasal organ (VNO) morphology varies markedly across primate taxa. Old World monkeys display no postnatal VNO. Humans and at least some apes retain a vestigial VNO during postnatal life, whereas the strepsirrhines and New World Monkeys present a morphologically well-defined VNO that, in many species, is presumed to function as an olfactory organ. Available microanatomical and behavioral studies suggest that VNO function in these species does not precisely duplicate that described in other mammalian taxa. The questions of which species retain a functional VNO and what functions they serve require inquiry along diverse lines but, to be functional, the vomeronasal epithelium must be neuronal and olfactory. We used immunohistochemistry to establish these criteria in six primate species. We compared the expression of two neuronal markers, neuron-specific beta-tubulin (BT) and protein gene product 9.5, and olfactory marker protein (OMP), a marker of mature olfactory sensory neurons, in paraffin-embedded VNO sections from two strepsirrhine and four haplorhine species, all of which retain morphologically well-defined VNOs during postnatal life. The infant Eulemur mongoz, adult Otolemur crassicaudatus, neonatal Leontopithicus rosalia, and adult Callithrix jacchus express all three proteins in their well-defined vomeronasal neuroepithelia. The infant Tarsius syrichta showed some BT and OMP immunoreactivity. We establish that two strepsirrhine species and at least some New World haplorhines have mature sensory neurons in the VNO. In contrast, at all ages examined, Saguinus geoffroyi VNO expresses these markers in only a few cells., ((c) 2004 Wiley-Liss, Inc.)

Published

2004

4. Ontogenetic observations on the vomeronasal organ in two species of tamarins using neuron-specific beta-tubulin III.

Author

Smith TD, Dennis JC, Bhatnagar KP, Bonar CJ, Burrows AM, and Morrison EE

Subjects

Age Factors, Animals, Cell Count, Immunohistochemistry, Nasal Mucosa anatomy & histology, Olfactory Receptor Neurons anatomy & histology, Olfactory Receptor Neurons metabolism, Saguinus growth & development, Species Specificity, Tubulin, Vomeronasal Organ growth & development, Animals, Newborn anatomy & histology, Models, Anatomic, Saguinus anatomy & histology, Vomeronasal Organ anatomy & histology

Abstract

Callitrichid primates (tamarins, marmosets) have extreme variation in the vomeronasal organ (VNO), including ontogenetic differences in the neuroepithelium and vomeronasal duct (VND) patency at birth. Such differences render the timing and extent of VNO maturation debatable in callitrichids, but no studies have used neuron-specific immunohistochemical markers to address this question. The present study compared the number of VNO epithelial cells that express immunoreactivity to neuron-specific beta-tubulin III (BT), VNO length, and VNO cross-sectional area between two species of tamarins (Leontopithecus rosalia and Saguinus geoffroyi) that differed in perinatal VND patency. Neonatal lemurs and adult marmosets and bushbabies were also examined for a comparison to species previously shown to have a relatively large amount of VNO neuroepithelium and patent VNDs. The head of each specimen was serially sectioned in the coronal plane. Based on known rostrocaudal start/stop points of the VNO, selected unstained sections were used for BT protocols and area measurement at three percentiles (25th, 50th, 75th) in each specimen. Each section was photographed and enlarged for cell counts and measurement of cross-sectional epithelial area. In each specimen, the number of BT(+) cells in the VNO was counted at each percentile and expressed as a number per mm(2). Results indicated that lemur VNOs had a dense population of BT(+) cells at birth, but the VNO was more varied in the tamarin species. S. geoffroyi had few or no BT(+) cells in VNOs of neonates, which had fused VNDs, but had an increased BT(+) population by 1 and 2 months postnatal age, when the VND was patent. Of the species with patent VNDs at birth, neonatal L. rosalia had a denser population of BT(+) cells compared to S. geoffroyi, though not to the degree seen in neonatal lemurs or adult marmosets and bushbabies. These findings show that BT immunohistochemistry is a useful comparative method for the study of VNOs in subadult primates. Since the quantity of nonsensory VNO epithelium varies substantially between species, epithelial area measurements may be misleading, and BT(+) cell counts appeared to be the best quantitative method for comparing receptor neuron numbers among primates. It is suggested that the greater BT(+) cell population in L. rosalia at all subadult stages examined reveals an earlier maturation of the neuroepithelium compared to S. geoffroyi. Further investigation should consider whether this may relate to a comparatively brief subadult ontogeny and early onset of adult behaviors in L. rosalia compared to other tamarins studied to date., (Copyright 2004 Wiley-Liss, Inc.)

Published

2004

5. CLIP-170 interacts with dynactin complex and the APC-binding protein EB1 by different mechanisms.

Author

Goodson HV, Skube SB, Stalder R, Valetti C, Kreis TE, Morrison EE, and Schroer TA

Subjects

Amino Acid Motifs, Amino Acid Sequence, Dynactin Complex, HeLa Cells, Humans, Microtubule-Associated Proteins genetics, Molecular Sequence Data, Mutagenesis, Site-Directed, Mutation, Neoplasm Proteins, Protein Structure, Tertiary, Microtubule-Associated Proteins metabolism

Abstract

CLIP-170 is a "cytoplasmic linker protein" implicated in endosome-microtubule interactions and in control of microtubule dynamics. CLIP-170 localizes dynamically to growing microtubule plus ends, colocalizing with the dynein activator dynactin and the APC-binding protein EB1. This shared "plus-end tracking" behavior suggests that CLIP-170 might interact with dynactin and/or EB1. We have used site-specific mutagenesis of CLIP-170 and a transfection/colocalization assay to address this question in mammalian tissue culture cells. Our results indicate that CLIP-170 interacts, directly or indirectly, with both dynactin and EB1. We find that the CLIP-170/dynactin interaction is mediated by the second metal binding motif of the CLIP-170 tail. In contrast, the CLIP-170/EB1 interaction requires neither metal binding motif. In addition, our experiments suggest that the CLIP-170/dynactin interaction occurs via the shoulder/sidearm subcomplex of dynactin and can occur in the cytosol (i.e., it does not require microtubule binding). These results have implications for the targeting of both dynactin and EB1 to microtubule plus ends. Our data suggest that the CLIP-170/dynactin interaction can target dynactin complex to microtubule plus ends, although dynactin likely also targets MT plus ends directly via the microtubule binding motif of the p150(Glued) subunit. We find that CLIP-170 mutants alter p150(Glued) localization without affecting EB1, indicating that EB1 can target microtubule plus ends independently of dynactin., (Copyright 2003 Wiley-Liss, Inc.)

Published

2003

6. Morphology of olfactory epithelium in humans and other vertebrates.

Author

Morrison EE and Costanzo RM

Subjects

Animals, Cilia physiology, Cilia ultrastructure, Humans, Olfactory Mucosa physiology, Sensory Receptor Cells physiology, Sensory Receptor Cells ultrastructure, Vertebrates physiology, Olfactory Mucosa ultrastructure, Vertebrates anatomy & histology

Abstract

Human olfactory epithelium is similar in organization and cell morphology to that of most vertebrate species. The epithelium has a pseudostratified columnar organization and consists of olfactory neurons, supporting and basal cells. Near the mucosal surface there are also microvillar cells. These cells have neuron-like features and may be chemoreceptors. Human olfactory epithelium is not a uniform sensory sheet. Patches of non-sensory tissue often appear in what was thought to be a purely olfactory region. The significance of these patches has not been determined, but they could reflect exposure to environment agents or changes that occur during the normal aging process. In order to better understand the human olfactory system, further knowledge of the normal structure is necessary. This review addresses the morphology of the human olfactory epithelium and the remarkable plasticity of the vertebrate olfactory system.

Published

1992

7. Morphology of the human olfactory epithelium.

Author

Morrison EE and Costanzo RM

Subjects

Humans, Microscopy, Electron, Scanning, Microvilli ultrastructure, Neurons cytology, Olfactory Mucosa cytology, Olfactory Mucosa innervation, Olfactory Mucosa ultrastructure

Abstract

The human olfactory epithelium has been previously studied with scanning electron microscopy; however, most studies have been limited to examining the epithelial surface. In an attempt to examine structures below the surface, we scanned epithelial fractures that occurred during tissue preparation. This made it possible to obtain unique three-dimensional images of cell profiles from the mucosal surface through the full depth of the epithelium. We examined supporting cells, olfactory neurons, basal cells, and a fourth cell type, the microvillar cell. Supporting cells had a microvillar surface and were in close contact with olfactory neurons and their processes. Olfactory neurons were primarily located in the middle and lower epithelial regions. Basal cells occurred alone or in clusters adjacent to the basal lamina. Microvillar cells were always observed in the upper epithelial region. They were flask- or pear-shaped, had a tuft of microvilli that extended into the nasal cavity, and a thin axon-like process that passed basally towards the lamina propria. This study represents the first comprehensive scanning electron microscopy examination of the human olfactory epithelium. Three-dimensional images obtained for each epithelial cell type allowed us to examine cell processes and their close contacts, especially between supporting cells and olfactory neurons. These results also revealed the irregular and patchy distribution of olfactory receptors within the human nasal cavity. Further studies that examine the detailed morphology of the human olfactory epithelium should provide a better understanding of the physiological mechanism and clinical disorders that affect olfactory function in humans.

Published

1990