Your search keyword '"Ekaterina Dadachova"' showing total 85 results

1. In Vitro and In Vivo Comparison of Random versus Site-Specific Conjugation of Bifunctional Chelating Agents to the CD33-Binding Antibody for Use in Alpha- and Beta-Radioimmunotherapy

Author

Kevin J. H. Allen, Connor Frank, Rubin Jiao, Mackenzie E. Malo, Michele Bello, Laura De Nardo, Laura Meléndez-Alafort, and Ekaterina Dadachova

Subjects

Chemistry, QD1-999

Published

2024

2. Radioimmunotherapy combating biofilm-associated infection in vitro

Author

Zijian Ye, Berend van der Wildt, F. Ruben H. A. Nurmohamed, J. Fred F. Hooning van Duyvenbode, Jos van Strijp, H. Charles Vogely, Marnix G. E. H. Lam, Ekaterina Dadachova, Harrie Weinans, Bart C. H. van der Wal, and Alex J. Poot

Subjects

radioimmunotherapy, Staphylococcus aureus, biofilm, antibodies, infection, wall teichoic acids, Medicine (General), R5-920

Abstract

BackgroundAddressing prosthetic joint infections poses a significant challenge within orthopedic surgery, marked by elevated morbidity and mortality rates. The presence of biofilms and infections attributed to Staphylococcus aureus (S. aureus) further complicates the scenario.ObjectiveTo investigate the potential of radioimmunotherapy as an innovative intervention to tackle biofilm-associated infections.MethodsOur methodology involved employing specific monoclonal antibodies 4497-IgG1, designed for targeting wall teichoic acids found on S. aureus and its biofilm. These antibodies were linked with radionuclides actinium-225 (225Ac) and lutetium-177 (177Lu) using DOTA as a chelator. Following this, we evaluated the susceptibility of S. aureus and its biofilm to radioimmunotherapy in vitro, assessing bacterial viability and metabolic activity via colony-forming unit enumeration and xylenol tetrazolium assays.ResultsBoth [225Ac]4497-IgG1 and [177Lu]4497-IgG1 exhibited a noteworthy dose-dependent reduction in S. aureus in planktonic cultures and biofilms over a 96-h exposure period, compared to non-specific antibody control groups. Specifically, doses of 7.4 kBq and 7.4 MBq of [225Ac]4497-IgG1 and [177Lu]4497-IgG1 resulted in a four-log reduction in planktonic bacterial counts. Within biofilms, 14.8 kBq of [225Ac]4497-IgG1 and 14.8 Mbq [177Lu]4497-IgG1 led to reductions of two and four logs, respectively.ConclusionOur findings underscore the effectiveness of [225Ac]4497-IgG1 and [177Lu]4497-IgG1 antibodies in exerting dose-dependent bactericidal effects against planktonic S. aureus and biofilms in vitro. This suggests that radioimmunotherapy might serve as a promising targeted treatment approach for combating S. aureus and its biofilm.

Published

2024

3. Comparative Molecular Characterization and Pharmacokinetics of IgG1-Fc and Engineered Fc Human Antibody Variants to Insulin-like Growth Factor 2 Receptor (IGF2R)

Author

Chandra B. Prabaharan, Sabeena Giri, Kevin J. H. Allen, Katrina E. M. Bato, Therese R. Mercado, Mackenzie E. Malo, Jorge L. C. Carvalho, Ekaterina Dadachova, and Maruti Uppalapati

Subjects

osteosarcoma (OS), insulin-like growth factor 2 receptor (IGF2R), monoclonal antibodies, neonatal Fc receptor (FcRn), radioimmunotherapy (RIT), Organic chemistry, QD241-441

Abstract

Novel therapeutic approaches are much needed for the treatment of osteosarcoma. Targeted radionuclide therapy (TRT) and radioimmunotherapy (RIT) are promising approaches that deliver therapeutic radiation precisely to the tumor site. We have previously developed a fully human antibody, named IF3, that binds to insulin-like growth factor 2 receptor (IGF2R). IF3 was used in TRT to effectively inhibit tumor growth in osteosarcoma preclinical models. However, IF3’s relatively short half-life in mice raised the need for improvement. We generated an Fc-engineered version of IF3, termed IF3δ, with amino acid substitutions known to enhance antibody half-life in human serum. In this study, we confirmed the specific binding of IF3δ to IGF2R with nanomolar affinity, similar to wild-type IF3. Additionally, IF3δ demonstrated binding to human and mouse neonatal Fc receptors (FcRn), indicating the potential for FcRn-mediated endocytosis and recycling. Biodistribution studies in mice showed a higher accumulation of IF3δ in the spleen and bone than wild-type IF3, likely attributed to abnormal spleen expression of IGF2R in mice. Therefore, the pharmacokinetics data from mouse xenograft models may not precisely reflect their behavior in canine and human patients. However, the findings suggest both IF3 and IF3δ as promising options for the RIT of osteosarcoma.

Published

2023

4. Image-Based Dosimetry in Dogs and Cross-Reactivity with Human Tissues of IGF2R-Targeting Human Antibody

Author

Kevin J. H. Allen, Ohyun Kwon, Matthew R. Hutcheson, Joseph J. Grudzinski, Stuart M. Cain, Frederic A. Cruz, Remitha M. Vinayakamoorthy, Ying S. Sun, Lindsay Fairley, Chandra B. Prabaharan, Ryan Dickinson, Valerie MacDonald-Dickinson, Maruti Uppalapati, Bryan P. Bednarz, and Ekaterina Dadachova

Subjects

IGF2R, osteosarcoma, image-based dosimetry RAPID, 89Zr, 177Lu, tissue cross-reactivity, Medicine, Pharmacy and materia medica, RS1-441

Abstract

Background: Osteosarcoma (OS) represents the most common primary bone tumor in humans and in companion dogs, being practically phenotypically identical. There is a need for effective treatments to extend the survival of patients with OS. Here, we examine the dosimetry in beagle dogs and cross-reactivity with human tissues of a novel human antibody, IF3, that targets the insulin growth factor receptor type 2 (IGF2R), which is overexpressed on OS cells, making it a candidate for radioimmunotherapy of OS. Methods: [89Zr]Zr-DFO-IF3 was injected into three healthy beagle dogs. PET/CT was conducted at 4, 24, 48, and 72 h. RAPID analysis was used to determine the dosimetry of [177Lu]Lu-CHXA”-IF3 for a clinical trial in companion dogs with OS. IF3 antibody was biotinylated, and a multitude of human tissues were assessed with immunohistochemistry. Results: PET/CT revealed that only the liver, bone marrow, and adrenal glands had high uptake. Clearance was initially through renal and hepatobiliary excretion in the first 72 h followed by primarily physical decay. RAPID analysis showed bone marrow to be the dose-limiting organ with a therapeutic range for 177Lu calculated to be 0.487–0.583 GBq. Immunohistochemistry demonstrated the absence of IGF2R expression on the surface of healthy human cells, thus suggesting that radioimmunotherapy with [177Lu]Lu-CHXA”-IF3 will be well tolerated. Conclusions: Image-based dosimetry has defined a safe therapeutic range for canine clinical trials, while immunohistochemistry has suggested that the antibody will not cross-react with healthy human tissues.

Published

2023

5. 225Ac‐labeled CD33‐targeting antibody reverses resistance to Bcl‐2 inhibitor venetoclax in acute myeloid leukemia models

Author

Ravendra Garg, Kevin J. H. Allen, Wojciech Dawicki, Eileen M. Geoghegan, Dale L. Ludwig, and Ekaterina Dadachova

Subjects

225Ac‐lintuzumab, acute myeloid leukemia, Bcl‐2, radioimmunotherapy, venetoclax, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

ABSTRACT Purpose Despite the availability of new drugs, many patients with acute myeloid leukemia (AML) do not achieve remission and outcomes remain poor. Venetoclax is a promising new therapy approved for use in combination with a hypomethylating agent or with low‐dose cytarabine for the treatment of newly diagnosed older AML patients or those ineligible for intensive chemotherapy. 225Actinium‐lintuzumab (225Ac‐lintuzumab) is a clinical stage radioimmunotherapy targeting CD33 that has shown evidence of single‐agent activity in relapsed/refractory AML. Increased expression of MCL‐1 is a mediator of resistance to venetoclax in cancer. Experimental design Here we investigated the potential for 225Ac‐lintuzumab‐directed DNA damage to suppress MCL‐1 levels as a possible mechanism of reversing resistance to venetoclax in two preclinical in vivo models of AML. Results We demonstrated that 225Ac‐lintuzumab in combination with venetoclax induced a synergistic increase in tumor cell killing compared to treatment with either drug alone in venetoclax‐resistant AML cell lines through both an induction of double‐stranded DNA breaks (DSBs) and depletion of MCL‐1 protein levels. Further, this combination led to significant tumor growth control and prolonged survival benefit in venetoclax‐resistant in vivo AML models. Conclusions There results suggest that the combination of 225Ac‐lintuzumab with venetoclax is a promising therapeutic strategy for the treatment of patients with venetoclax‐resistant AML. Clinical trial of this combination therapy (NCT03867682) is currently ongoing.

Published

2021

6. Transcriptomic and genomic changes associated with radioadaptation in Exophiala dermatitidis

Author

Mackenzie E. Malo, Zachary Schultzhaus, Connor Frank, Jillian Romsdahl, Zheng Wang, and Ekaterina Dadachova

Subjects

Fungi, Melanin, Ionizing radiation, Transcriptome, Radioadaptation, Biotechnology, TP248.13-248.65

Abstract

Melanized fungi have been isolated from some of the harshest radioactive environments, and their ability to thrive in these locations is in part due to the pigment melanin. Melanin imparts a selective advantage to fungi by providing a physical shield, a chemical shield, and possibly a signaling mechanism. In previous work we demonstrated that protracted exposure of the melanized yeast Exophiala dermatitidis to mixed alpha-, beta-, and gamma-emitting radiation resulted in an adapted strain able to mount a unique response to ionizing radiation in the environment in a melanin-dependent fashion. By exploring the genome and transcriptome of this adapted melanized strain relative to a non-irradiated control we determined the altered response was transcriptomic in nature, as whole genome sequencing revealed limited variation. Transcriptomic analysis indicated that of the adapted isolates analyzed, two lineages existed: one like the naïve, non-adapted strain, and one with a unique transcriptomic signature that exhibited downregulation of metabolic processes, and upregulation of translation-associated genes. Analysis of differential gene expression in the adapted strain showed an overlap in response between the control conditions and reactive oxygen species conditions, whereas exposure to an alpha particle source resulted in a robust downregulation of metabolic processes and upregulation of DNA replication and repair genes, and RNA metabolic processes. This suggest previous exposure to radiation primes the fungus to respond to subsequent exposures in a unique way. By exploring this unique response, we have expanded our knowledge of how melanized fungi interact with and respond to ionizing radiation in their environment.

Published

2021

7. Highlights of the Latest Developments in Radiopharmaceuticals for Infection Imaging and Future Perspectives

Author

Ekaterina Dadachova and Drauzio E. N. Rangel

Subjects

infection imaging, antibiotics, anti-fungals, antimicrobial peptides, antibodies, HIV, Medicine (General), R5-920

Abstract

COVID-19 pandemic has heightened the interest toward diagnosis and treatment of infectious diseases. Nuclear medicine with its powerful scintigraphic, single photon emission computer tomography (SPECT) and positron emission tomography (PET) imaging modalities has always played an important role in diagnosis of infections and distinguishing them from the sterile inflammation. In addition to the clinically available radiopharmaceuticals there has been a decades-long effort to develop more specific imaging agents with some examples being radiolabeled antibiotics and antimicrobial peptides for bacterial imaging, radiolabeled anti-fungals for fungal infections imaging, radiolabeled pathogen-specific antibodies and molecular engineered constructs. In this opinion piece, we would like to discuss some examples of the work published in the last decade on developing nuclear imaging agents for bacterial, fungal, and viral infections in order to generate more interest among nuclear medicine community toward conducting clinical trials of these novel probes, as well as toward developing novel radiotracers for imaging infections.

Published

2022

8. Human monoclonal antibodies against Staphylococcus aureus surface antigens recognize in vitro and in vivo biofilm

Author

Lisanne de Vor, Bruce van Dijk, Kok van Kessel, Jeffrey S Kavanaugh, Carla de Haas, Piet C Aerts, Marco C Viveen, Edwin C Boel, Ad C Fluit, Jakub M Kwiecinski, Gerard C Krijger, Ruud M Ramakers, Freek J Beekman, Ekaterina Dadachova, Marnix GEH Lam, H Charles Vogely, Bart CH van der Wal, Jos AG van Strijp, Alexander R Horswill, Harrie Weinans, and Suzan HM Rooijakkers

Subjects

Staphylococcus aureus, biofilm, monoclonal antibodies, Medicine, Science, Biology (General), QH301-705.5

Abstract

Implant-associated Staphylococcus aureus infections are difficult to treat because of biofilm formation. Bacteria in a biofilm are often insensitive to antibiotics and host immunity. Monoclonal antibodies (mAbs) could provide an alternative approach to improve the diagnosis and potential treatment of biofilm-related infections. Here, we show that mAbs targeting common surface components of S. aureus can recognize clinically relevant biofilm types. The mAbs were also shown to bind a collection of clinical isolates derived from different biofilm-associated infections (endocarditis, prosthetic joint, catheter). We identify two groups of antibodies: one group that uniquely binds S. aureus in biofilm state and one that recognizes S. aureus in both biofilm and planktonic state. Furthermore, we show that a mAb recognizing wall teichoic acid (clone 4497) specifically localizes to a subcutaneously implanted pre-colonized catheter in mice. In conclusion, we demonstrate the capacity of several human mAbs to detect S. aureus biofilms in vitro and in vivo.

Published

2022

9. Effects of Melanized Bacteria and Soluble Melanin on the Intestinal Homeostasis and Microbiome In Vivo

Author

Yong-guo Zhang, Mackenzie E. Malo, Tanya Tschirhart, Yinglin Xia, Zheng Wang, Ekaterina Dadachova, and Jun Sun

Subjects

E. coli Nissle, intestine, melanin, melanized bacteria, microbiome, probiotics, Chemical technology, TP1-1185

Abstract

Radiation damage is associated with inflammation and immunity in the intestinal mucosa, including gut microbiota. Melanin has a unique capacity to coordinate a biological reaction in response to environmental stimuli, such as radiation exposure. Thus, melanin and melanized microbes have potential to be used for mitigation of injury induced by radiation. The purpose of the current study is to examine the safety of these agents for future targeting gut microbiome to prevent radiation-induced injury. We administered mice with soluble allomelanin and observed its effect on the intestinal physiology and body weight. We then established a melanized bacterial strain in probiotic E. coli Nissle. We measured the body weight of the mice treated with melanized E. coli Nissle. We showed the enhanced bacterial abundance and colonization of the melanized bacteria E. coli Nissle in the intestine. Melanized E. coli Nissle colonized the colon in less than 3 h and showed consistent colonization over 24 h post one oral gavage. We did not find significant changes of bodyweight in the mice treated with melanized bacteria. We did not observe any inflammation in the intestine. These results demonstrate the safety of soluble melanin and melanin-producing bacteria and will support the future studies to treat radiation-induced injuries and restore dysbiosis.

Published

2022

10. Monoclonal Antibodies Against Human Papillomavirus E6 and E7 Oncoproteins Inhibit Tumor Growth in Experimental Cervical Cancer

Author

Zewei Jiang, Joseph Albanese, Joshua Kesterson, Joshua Warrick, Rouzan Karabakhtsian, Ekaterina Dadachova, and Rébécca Phaëton

Subjects

Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

Nearly all cases of cervical cancer are initiated by persistent infection with high-risk strains of human papillomavirus (hr-HPV). When hr-HPV integrates into the host genome, the constitutive expression of oncogenic HPV proteins E6 and E7 function to disrupt p53 and retinoblastoma regulation of cell cycle, respectively, to favor malignant transformation. HPV E6 and E7 are oncogenes found in over 99% of cervical cancer, they are also expressed in pre-neoplastic stages making these viral oncoproteins attractive therapeutic targets. Monoclonal antibodies (mAbs) represent a novel potential approach against the actions of hr-HPV E6 and E7 oncoproteins.In this report, we describe the utilization of anti-HPV E6 and HPV E7 mAbs in an experimental murine model of human cervical cancer tumors. We used differential dosing strategies of mAbs C1P5 (anti-HPV 16 E6) and TVG701Y (anti-HPV E7) administered via intraperitoneal or intratumoral injections. We compared mAbs to the action of chemotherapeutic agent Cisplatin and demonstrated the capacity of mAbs to significantly inhibit tumor growth. Furthermore, we investigated the contribution of the immune system and found increased complement deposition in both C1P5 and TVG701Y treated tumors compared to irrelevant mAb therapy. Taken together, the results suggest that anti-HPV E6 and E7 mAbs exert inhibition of tumor growth in a viral-specific manner and stimulate an immune response that could be exploited for an additional treatment options for patients. Keywords: cervical cancer, monoclonal antibodies, HPV E6 and E7, immunotherapy, nude mice

Published

2019

11. Evaluation of novel highly specific antibodies to cancer testis antigen Centrin‐1 for radioimmunoimaging and radioimmunotherapy of pancreatic cancer

Author

Rubin Jiao, Kevin J. H. Allen, Mackenzie E. Malo, Muath Helal, Zewei Jiang, Karishma Smart, Susan V. Buhl, David Rickles, Ruth A. Bryan, and Ekaterina Dadachova

Subjects

177Lutetium, 213Bismuth, centrin1, pancreatic adenocarcinoma, radioimmunotherapy, SPECT/CT imaging, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

Abstract Background Pancreatic ductal adenocarcinoma (PDAC) accounts for >90% of pancreatic malignancies, and has median survival of

Published

2019

12. In Vitro and In Vivo Characterization of 89Zirconium-Labeled Lintuzumab Molecule

Author

Kevin J. H. Allen, Rubin Jiao, Jason Li, Denis R. Beckford-Vera, and Ekaterina Dadachova

Subjects

lintuzumab, 89Zirconium, positron emission tomography, acute myeloid leukemia, Organic chemistry, QD241-441

Abstract

Objective: Positron emission tomography (PET) imaging is a powerful non-invasive method to determine the in vivo behavior of biomolecules. Determining biodistribution and pharmacokinetic (PK) properties of targeted therapeutics can enable a better understanding of in vivo drug mechanisms such as tumor uptake, off target accumulation and clearance. Zirconium-89 (89Zr) is a readily available tetravalent PET-enabling radiometal that has been used to evaluate the biodistribution and PK of monoclonal antibodies. In the current study, we performed in vitro and in vivo characterization of 89Zr-lintuzumab, a radiolabeled anti-CD33 antibody, as a model to evaluate the in vivo binding properties in preclinical models of AML. Methods: Lintuzumab was conjugated to p-SCN-Bn-deferoxamine (DFO) and labeled with 89Zr using a 5:1 µCi:µg specific activity at 37 °C for 1h. The biological activity of 89Zr-lintuzumab was evaluated in a panel of CD33 positive cells using flow cytometry. Fox Chase SCID mice were injected with 2 × 106 OCI-AML3 cells into the right flank. After 12 days, a cohort of mice (n = 4) were injected with 89Zr-lintuzumab via tail vein. PET/CT scans of mice were acquired on days 1, 2, 3 and 7 post 89Zr-lintuzumab injection. To demonstrate 89Zr-lintuzumab specific binding to CD33 expressing tumors in vivo, a blocking study was performed. This cohort of mice (n = 4) was injected with native lintuzumab and 24 h later 89Zr-lintuzumab was administered. This group was imaged 3 and 7 days after injection of 89Zr-lintuzumab. A full ex vivo biodistribution study on both cohorts was performed on day 7. The results from the PET image and ex vivo biodistribution studies were compared. Results: Lintuzumab was successfully radiolabeled with 89Zr resulting in a 99% radiochemical yield. The 89Zr-lintuzumab radioconjugate specifically binds CD33 positive cells in a similar manner to native lintuzumab as observed by flow cytometry. PET imaging revealed high accumulation of 89Zr-lintuzumab in OCI-AML3 tumors within 24h post-injection of the radioconjugate. The 89Zr-lintuzumab high tumor uptake remains for up to 7 days. Tumor analysis of the PET data using volume of interest (VOI) showed significant blocking of 89Zr-lintuzumab in the group pre-treated with native lintuzumab (pre-blocked group), thus indicating specific targeting of CD33 on OCI-AML3 cells in vivo. The tumor uptake findings from the PET imaging study are in agreement with those from the ex vivo biodistribution results. Conclusions: PET imaging of 89Zr-lintuzumab shows high specific uptake in CD33 positive human OCI-AML3 tumors. The results from the image study agree with the observations from the ex vivo biodistribution study. Our findings collectively suggest that PET imaging using 89Zr-lintuzumab could be a powerful drug development tool to evaluate binding properties of anti-CD33 monoclonal antibodies in preclinical cancer models.

Published

2022

13. Radioimmunotherapy Targeting IGF2R on Canine-Patient-Derived Osteosarcoma Tumors in Mice and Radiation Dosimetry in Canine and Pediatric Models

Author

Jaline Broqueza, Chandra B. Prabaharan, Kevin J. H. Allen, Rubin Jiao, Darrell R. Fisher, Ryan Dickinson, Valerie MacDonald-Dickinson, Maruti Uppalapati, and Ekaterina Dadachova

Subjects

osteosarcoma, IGF2R, radioimmunotherapy, canine-patient-derived Gracie tumors, human dosimetry, canine dosimetry, Medicine, Pharmacy and materia medica, RS1-441

Abstract

Background: Osteosarcoma (OS) has an overall patient survival rate of ~70% with no significant improvements in the last two decades, and novel effective treatments are needed. OS in companion dogs is phenotypically close to human OS, which makes a comparative oncology approach to developing new treatments for OS very attractive. We have recently created a novel human antibody, IF3 to IGF2R, which binds to this receptor on both human and canine OS tumors. Here, we evaluated the efficacy and safety of radioimmunotherapy with 177Lu-labeled IF3 of mice bearing canine-patient-derived tumors and performed canine and human dosimetry calculations. Methods: Biodistribution and microSPECT/CT imaging with 111In-IF3 was performed in mice bearing canine OS Gracie tumors, and canine and human dosimetry calculations were performed based on these results. RIT of Gracie-tumor-bearing mice was completed with 177Lu-IF3. Results: Biodistribution and imaging showed a high uptake of 111In-IF3 in the tumor and spleen. Dosimetry identified the tumor, spleen and pancreas as the organs with the highest uptake. RIT was very effective in abrogating tumor growth in mice with some spleen-associated toxicity. Conclusions: These results demonstrate that RIT with 177Lu-IF3 targeting IGF2R on experimental canine OS tumors effectively decreases tumor growth. However, because of the limitations of murine models, careful evaluation of the possible toxicity of this treatment should be performed via nuclear imaging and image-based dosimetry in healthy dogs before clinical trials in companion dogs with OS can be attempted.

Published

2021

14. Radioimmunotherapy of Blastomycosis in a Mouse Model With a (1→3)-β-Glucans Targeting Antibody

Author

Muath Helal, Kevin J. H. Allen, Bruce van Dijk, Joshua D. Nosanchuk, Elisabeth Snead, and Ekaterina Dadachova

Subjects

radioimmunotherapy, Blastomyces dermatitidis, (1→3)-β-glucan, mouse model, 213Bismuth, Microbiology, QR1-502

Abstract

Invasive fungal infections (IFI) cause devastating morbidity and mortality, with the number of IFIs more than tripling since 1979. Our laboratories were the first to demonstrate that radiolabeled microorganism-specific monoclonal antibodies are highly effective for treatment of experimental fungal, bacterial and viral infections. Later we proposed to utilize surface expressed pan-antigens shared by major IFI-causing pathogens such as beta-glucans as RIT targets. Here we evaluated in vivo RIT targeting beta-glucan in Blastomyces dermatitidis which causes serious infections in immunocompromised and immunocompetent individuals and in companion dogs. B. dermatitidis cells were treated with the 400-2 antibody to (1→3)-β-glucans radiolabeled with the beta-emitter 177Lutetium (177Lu) and alpha-emitter 213Bismuth (213Bi) and the efficacy of cell kill was determined by colony forming units (CFUs). To determine the antigen-specific localization of the 400-2 antibody in vivo, C57BL6 mice were infected intratracheally with 2 × 105B. dermatitidis cells and given 111In-400-2 antibody 24 h later. To evaluate the killing of B. dermatitidis cells with RIT, intratracheally infected mice were treated with 150 μCi 213Bi-400-2 and their lungs analyzed for CFUs 96 h post-infection. 213Bi-400-2 proved to be more effective in killing B. dermatitidis cells in vitro than 177Lu-400-2. Three times more 111In-400-2 accumulated in the lungs of infected mice, than in the non-infected ones. 213Bi-400-2 lowered the fungal burden in the lungs of infected mice more than 2 logs in comparison with non-treated infected controls. In conclusion, our results demonstrate the ability of an anti-(1-3)-beta-D-glucan antibody armed with an alpha-emitter 213Bi to selectively kill B. dermatitidis cells in vitro and in vivo. These first in vivo results of the effectiveness of RIT targeting pan-antigens on fungal pathogens warrant further investigation.

Published

2020

15. Daratumumab-225Actinium conjugate demonstrates greatly enhanced antitumor activity against experimental multiple myeloma tumors

Author

Wojciech Dawicki, Kevin J.H. Allen, Rubin Jiao, Mackenzie E. Malo, Muath Helal, Mark S. Berger, Dale L. Ludwig, and Ekaterina Dadachova

Subjects

multiple myeloma, daratumumab, 225actinium, microspect/ct, radioimmunotherapy, Immunologic diseases. Allergy, RC581-607, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, RC254-282

Abstract

Daratumumab is an anti-CD38 directed monoclonal antibody approved for the treatment of multiple myeloma (MM) and functions primarily via Fc-mediated effector mechanisms such as complement-dependent cytotoxicity (CDC), antibody-dependent cell cytotoxicity (ADCC), antibody-dependent cellular phagocytosis, and T-cell activation. However, not all patients respond to daratumumab therapy and management of MM remains challenging. Radioimmunotherapy with alpha particle-emitting radionuclides represents a promising approach to significantly enhance the potency of therapeutic antibodies in cancer treatment. Here we report the results of mechanistic and feasibility studies using daratumumab radiolabeled with an alpha-emitter 225Actinium for therapy of MM. CD38-positivelymphoma Daudi cell line and MM cell lines KMS-28BM and KMS-28PE were treated in vitro with 225Ac-daratumumab. 225Ac-daratumumab Fc-functional properties were assessed with C1q binding and ADCC assays. The pharmacokinetics and tumor uptake of 111In-daratumumab in Daudi tumor-bearing severe combined immunodeficiency (SCID) mice were measured with microSPECT/CT. The therapeutic effects of 225Ac-daratumumab on Daudi and KSM28BM tumors in mice and treatment side effects were evaluated for 50 days posttreatment. The safety of 225Ac-labeled antimurine CD38 mAb in immunocompetent mice was also evaluated. 225Ac-daratumumab efficiently and specifically killed CD38-positive tumor cells in vitro, while its complement binding and ADCC functions remained unaltered. MicroSPECT/CT imaging demonstrated fast clearance of the radiolabeled daratumumab from the circulation and tissues, but prolonged retention in the tumor up to 10 days. Therapy and safety experiments with 225Ac-daratumumab showed a significant increase in the antitumor potency in comparison to naked antibody without any significant side effects. Our results highlight the potential of targeting alpha-emitters to tumors as a therapeutic approach and suggest that 225Ac-daratumumab may be a promising therapeutic strategy for the treatment of hematologic malignancies.

Published

2019

16. Safety Evaluation of an Alpha-Emitter Bismuth-213 Labeled Antibody to (1→3)-β-Glucan in Healthy Dogs as a Prelude for a Trial in Companion Dogs with Invasive Fungal Infections

Author

Muath Helal, Kevin J. H. Allen, Hilary Burgess, Rubin Jiao, Mackenzie E. Malo, Matthew Hutcheson, Ekaterina Dadachova, and Elisabeth Snead

Subjects

radioimmunotherapy, bismuth-213, invasive fungal infections, 1-3-beta-glucan, dogs, Organic chemistry, QD241-441

Abstract

Background: With the limited options available for therapy to treat invasive fungal infections (IFI), radioimmunotherapy (RIT) can potentially offer an effective alternative treatment. Microorganism-specific monoclonal antibodies have shown promising results in the experimental treatment of fungal, bacterial, and viral infections, including our recent and encouraging results from treating mice infected with Blastomyces dermatitidis with 213Bi-labeled antibody 400-2 to (1→3)-β-glucan. In this work, we performed a safety study of 213Bi-400-2 antibody in healthy dogs as a prelude for a clinical trial in companion dogs with acquired invasive fungal infections and later on in human patients with IFI. Methods: Three female beagle dogs (≈6.1 kg body weight) were treated intravenously with 155.3, 142.5, or 133.2 MBq of 213Bi-400-2 given as three subfractions over an 8 h period. RBC, WBC, platelet, and blood serum biochemistry parameters were measured periodically for 6 months post injection. Results: No significant acute or long-term side effects were observed after RIT injections; only a few parameters were mildly and transiently outside reference change value limits, and a transient atypical morphology was observed in the circulating lymphocyte population of two dogs. Conclusions: These results demonstrate the safety of systemic 213Bi-400-2 administration in dogs and provide encouragement to pursue evaluation of RIT of IFI in companion dogs.

Published

2020

17. Comparative Radioimmunotherapy of Experimental Melanoma with Novel Humanized Antibody to Melanin Labeled with 213Bismuth and 177Lutetium

Author

Kevin J. H. Allen, Rubin Jiao, Mackenzie E. Malo, Connor Frank, Darrell R. Fisher, David Rickles, and Ekaterina Dadachova

Subjects

radioimmunotherapy, humanized antibody, melanin, B16-F10 melanoma, 213Bismuth, 177Lutetium, Pharmacy and materia medica, RS1-441

Abstract

Melanoma is a cancer with increasing incidence and there is a need for alternatives to immunotherapy within effective approaches to treatment of metastatic melanoma. We performed comparative radioimmunotherapy (RIT) of experimental B16-F10 melanoma with novel humanized IgG to melanin h8C3 labeled with a beta emitter, 177Lu, and an alpha-emitter, 213Bi, as well as biodistribution, microSPECT/CT imaging, and mouse and human dosimetry calculations. microSPECT/CT imaging showed that a humanized antibody that targets “free” melanin in the tumor microenvironment had high tumor uptake in B16F10 murine melanoma in C57Bl/6 mice, with little to no uptake in naturally melanized tissues. Extrapolation of the mouse dosimetry data to an adult human demonstrated that doses delivered to major organs and the whole body by 177Lu-h8C3 would be approximately two times higher than those delivered by 213Bi-h8C3, while the doses to the tumor would be almost similar. RIT results indicated that 213Bi-h8C3 was more effective in slowing down the tumor growth than 177Lu-h8C3, while both radiolabeled antibodies did not produce significant hematologic or systemic side effects. We concluded that h8C3 antibody labeled with 213Bi is a promising reagent for translation into a clinical trial in patients with metastatic melanoma.

Published

2019

18. Combination of anti-retroviral drugs and radioimmunotherapy specifically kills infected cells from HIV infected individuals

Author

Dina Tsukrov, Alicia McFarren, Alfred Morgenstern, Frank Bruchertseifer, Eugene Dolce, Miroslaw K Gorny, Susan Zolla-Pazner, Joan W Berman, Ellie Schoenbaum, Barry S Zingman, Arturo Casadevall, and Ekaterina Dadachova

Subjects

HIV, Patients, Radioimmunotherapy, gp41, antiretroviral therapy, 213Bismuth, Medicine (General), R5-920

Abstract

Eliminating virally infected cells is an essential component of any HIV eradication strategy. Radioimmunotherapy (RIT), a clinically established method for killing cells using radiolabeled antibodies, was recently applied to target HIV-1 gp41 antigen expressed on the surface of infect-ed cells. Since gp41 expression by infected cells is likely down-regulated in patients on an-tiretroviral therapy (ART), we evaluated the ability of RIT to kill ART-treated infected cells us-ing both in vitro models and lymphocytes isolated from HIV-infected subjects. Human peripheral blood mononuclear cells (PBMCs) were infected with HIV and cultured in the presence of two clinically relevant ART combinations. Scatchard analysis of the 2556 human monoclonal anti-body to HIV gp41 binding to the infected and ART-treated cells demonstrated sufficient residual expression of gp41 on the cell surface to warrant subsequent RIT. This is the first time the quantification of gp41 post-ART is being reported. Cells were then treated with Bismuth-213-labeled 2556 antibody. conjugated to the human monoclonal antibody 2556, which binds to HIV gp41. Cell survival was quantified by Trypan blue and residual viremia by p24 ELISA. Cell surface gp41 expression was assessed by Scatchard analysis. The experiments were repeated using PBMCs isolated from blood specimens obtained from 15 HIV-infected individuals: ten on ART and five ART-naive. We found that 213Bi-2556 killed ART-treated infected PBMCs and reduced viral production to undetectable levels. ART and RIT co-treatment was more effective at reducing viral load in vitro than either therapy alone, indicating that gp41 expression under ART was sufficient to allow 213Bi-2556 to deliver cytocidal doses of radiation to infected cells. This study provides proof of concept that 213Bi-2556 may represent an innovative and effective targeting method for killing HIV-infected cells treated with ART, and supports continued development of 213Bi-2556 for co-administration with ART towards an HIV eradication strategy.

Published

2016

19. Biodistribution of a Radiolabeled Antibody in Mice as an Approach to Evaluating Antibody Pharmacokinetics

Author

Kevin J. H. Allen, Rubin Jiao, Mackenzie E. Malo, Connor Frank, and Ekaterina Dadachova

Subjects

pharmacokinetics, antibodies, radiolabeling, biodistribution, mouse models, Pharmacy and materia medica, RS1-441

Abstract

(1) Background: Monoclonal antibodies are used in the treatment of multiple conditions including cancer, autoimmune disorders, and infectious diseases. One of the initial steps in the selection of an antibody candidate for further pre-clinical development is determining its pharmacokinetics in small animal models. The use of mass spectrometry and other techniques to determine the fate of these antibodies is laborious and expensive. Here we describe a straightforward and highly reproducible methodology for utilizing radiolabeled antibodies for pharmacokinetics studies. (2) Methods: Commercially available bifunctional linker CHXA„ and 111Indium radionuclide were used. A melanin-specific chimeric antibody A1 and an isotype matching irrelevant control A2 were conjugated with the CHXA„, and then radiolabeled with 111In. The biodistribution was performed at 4 and 24 h time points in melanoma tumor-bearing and healthy C57BL/6 female mice. (3) The biodistribution of the melanin-binding antibody showed the significant uptake in the tumor, which increased with time, and very low uptake in healthy melanin-containing tissues such as the retina of the eye and melanized skin. This biodistribution pattern in healthy tissues was very close to that of the isotype matching control antibody. (4) Conclusions: The biodistribution experiment allows us to assess the pharmacokinetics of both antibodies side by side and to make a conclusion regarding the suitability of specific antibodies for further development.

Published

2018

20. Quantitative Modeling of Microbial Population Responses to Chronic Irradiation Combined with Other Stressors.

Author

Igor Shuryak and Ekaterina Dadachova

Subjects

Medicine, Science

Abstract

Microbial population responses to combined effects of chronic irradiation and other stressors (chemical contaminants, other sub-optimal conditions) are important for ecosystem functioning and bioremediation in radionuclide-contaminated areas. Quantitative mathematical modeling can improve our understanding of these phenomena. To identify general patterns of microbial responses to multiple stressors in radioactive environments, we analyzed three data sets on: (1) bacteria isolated from soil contaminated by nuclear waste at the Hanford site (USA); (2) fungi isolated from the Chernobyl nuclear-power plant (Ukraine) buildings after the accident; (3) yeast subjected to continuous γ-irradiation in the laboratory, where radiation dose rate and cell removal rate were independently varied. We applied generalized linear mixed-effects models to describe the first two data sets, whereas the third data set was amenable to mechanistic modeling using differential equations. Machine learning and information-theoretic approaches were used to select the best-supported formalism(s) among biologically-plausible alternatives. Our analysis suggests the following: (1) Both radionuclides and co-occurring chemical contaminants (e.g. NO2) are important for explaining microbial responses to radioactive contamination. (2) Radionuclides may produce non-monotonic dose responses: stimulation of microbial growth at low concentrations vs. inhibition at higher ones. (3) The extinction-defining critical radiation dose rate is dramatically lowered by additional stressors. (4) Reproduction suppression by radiation can be more important for determining the critical dose rate, than radiation-induced cell mortality. In conclusion, the modeling approaches used here on three diverse data sets provide insight into explaining and predicting multi-stressor effects on microbial communities: (1) the most severe effects (e.g. extinction) on microbial populations may occur when unfavorable environmental conditions (e.g. fluctuations of temperature and/or nutrient levels) coincide with radioactive contamination; (2) an organism's radioresistance and bioremediation efficiency in rich laboratory media may be insufficient to carry out radionuclide bioremediation in the field--robustness against multiple stressors is needed.

Published

2016

21. Mathematical modeling predicts enhanced growth of X-ray irradiated pigmented fungi.

Author

Igor Shuryak, Ruth A Bryan, Joshua D Nosanchuk, and Ekaterina Dadachova

Subjects

Medicine, Science

Abstract

Ionizing radiation is known for its cytotoxic and mutagenic properties. However, recent evidence suggests that chronic sub-lethal irradiation stimulates the growth of melanin-pigmented (melanized) fungi, supporting the hypothesis that interactions between melanin and ionizing photons generate energy useful for fungal growth, and/or regulate growth-promoting genes. There are no quantitative models of how fungal proliferation is affected by ionizing photon energy, dose rate, and presence versus absence of melanin on the same genetic background. Here we present such a model, which we test using experimental data on melanin-modulated radiation-induced proliferation enhancement in the fungus Cryptococcus neoformans, exposed to two different peak energies (150 and 320 kVp) over a wide range of X-ray dose rates. Our analysis demonstrates that radiation-induced proliferation enhancement in C. neoformans behaves as a binary "on/off" phenomenon, which is triggered by dose rates 5000 mGy/h. Proliferation enhancement of irradiated cells compared with unirradiated controls occurs at both X-ray peak energies, but its magnitude is modulated by X-ray peak energy and cell melanization. At dose rates

Published

2014

22. Pre-clinical evaluation of a 213Bi-labeled 2556 antibody to HIV-1 gp41 glycoprotein in HIV-1 mouse models as a reagent for HIV eradication.

Author

Ekaterina Dadachova, Scott G Kitchen, Gregory Bristol, Gayle Cocita Baldwin, Ekaterina Revskaya, Cyril Empig, George B Thornton, Miroslaw K Gorny, Susan Zolla-Pazner, and Arturo Casadevall

Subjects

Medicine, Science

Abstract

Any strategy for curing HIV infection must include a method to eliminate viral-infected cells. Based on our earlier proof-of-principle results targeting HIV-1 infected cells with radiolabeled antibody (mAb) to gp41 viral antigen, we embarked on identifying a suitable candidate mAb for preclinical development.Among the several human mAbs to gp41 tested, mAb 2556 was found to have high affinity, reactivity with multimeric forms of gp41 present on both the surface of virus particles and cells expressing HIV-1 Env, and recognition of a highly conserved epitope of gp41 shared by all HIV-1 subtypes. Also, mAb 2556 was the best in competition with HIV-1+ serum antibodies, which is an extremely important consideration for efficacy in the treatment of HIV patients. When radiolabeled with alpha-emitting radionuclide 213-Bismuth ((213)Bi) - (213)Bi-2556 efficiently and specifically killed ACH-2 human lymphocytes chronically infected with HIV-1, and HIV-1 infected human peripheral blood mononuclear cells (hPBMCs). The number of binding sites for (213)Bi-2556 on the surface of the infected cells was >10(6). The in vivo experiments were performed in two HIV-1 mouse models--splenic and intraperitoneal. In both models, the decrease in HIV-1 infected hPBMCs from the spleens and peritoneum, respectively, was dose-dependent with the most pronounced killing of hPBMCs observed in the 100 µCi (213)Bi-2556 group (P = 0.01). Measurement of the blood platelet counts and gross pathology of the treated mice demonstrated the lack of toxicity for (213)Bi-2556.We describe the preclinical development of a novel radiolabeled mAb reagent that could potentially be part of an HIV eradication strategy that is ready for translation into the clinic as the next step in its development. As viral antigens are very different from "self" human antigens - this approach promises high selectivity, increased efficacy and low toxicity, especially in comparison to immunotoxins.

Published

2012

23. Correction: Pre-Clinical Evaluation of a Bi-Labeled 2556 Antibody to HIV-1 gp41 Glycoprotein in HIV-1 Mouse Models as a Reagent for HIV Eradication.

Author

Ekaterina Dadachova, Scott G. Kitchen, Gregory Bristol, Gayle Cocita Baldwin, Ekaterina Revskaya, Cyril Empig, George B. Thornton, Miroslaw K. Gorny, Susan Zolla-Pazner, and Arturo Casadevall

Subjects

Medicine, Science

Published

2012

24. Detection of urinary excreted fungal galactomannan-like antigens for diagnosis of invasive aspergillosis.

Author

Simon F Dufresne, Kausik Datta, Xinming Li, Ekaterina Dadachova, Janet F Staab, Thomas F Patterson, Marta Feldmesser, and Kieren A Marr

Subjects

Medicine, Science

Abstract

Mortality associated with invasive aspergillosis (IA) remains high, partly because of delayed diagnosis. Detection of microbial exoantigens, released in serum and other body fluids during infection, may help timely diagnosis. In course of IA, Aspergillus galactomannan (GM), a well established polysaccharide biomarker, is released in body fluids including urine. Urine is an abundant, safely collected specimen, well-suited for point-of-care (POC) testing, which could play an increasing role in screening for early disease. Our main objective was to demonstrate GM antigenuria as a clinically relevant biological phenomenon in IA and establish proof-of-concept that it could be translated to POC diagnosis. Utilizing a novel IgM monoclonal antibody (MAb476) that recognizes GM-like antigens from Aspergillus and other molds, we demonstrated antigenuria in an experimental animal IA model (guinea pig), as well as in human patients. In addition, we investigated the chemical nature of the urinary excreted antigen in human samples, characterized antigen detection in urine by immunoassays, described a putative assay inhibitor in urine, and indicated means of alleviation of the inhibition. We also designed and used a lateral flow immunochromatographic assay to detect urinary excreted antigen in a limited number of IA patient urine samples. In this study, we establish that POC diagnosis of IA based on urinary GM detection is feasible. Prospective studies will be necessary to establish the performance characteristics of an optimized device and define its optimal clinical use.

Published

2012

25. Protection of melanized Cryptococcus neoformans from lethal dose gamma irradiation involves changes in melanin's chemical structure and paramagnetism.

Author

Abdelahad Khajo, Ruth A Bryan, Matthew Friedman, Richard M Burger, Yan Levitsky, Arturo Casadevall, Richard S Magliozzo, and Ekaterina Dadachova

Subjects

Medicine, Science

Abstract

Certain fungi thrive in highly radioactive environments including the defunct Chernobyl nuclear reactor. Cryptococcus neoformans (C. neoformans), which uses L-3,4-dihydroxyphenylalanine (L-DOPA) to produce melanin, was used here to investigate how gamma radiation under aqueous aerobic conditions affects the properties of melanin, with the aim of gaining insight into its radioprotective role. Exposure of melanized fungal cell in aqueous suspensions to doses of γ-radiation capable of killing 50 to 80% of the cells did not lead to a detectable loss of melanin integrity according to EPR spectra of melanin radicals. Moreover, upon UV-visible (Xe-lamp) illumination of melanized cells, the increase in radical population was unchanged after γ-irradiation. Gamma-irradiation of frozen cell suspensions and storage of samples for several days at 77 K however, produced melanin modification noted by a reduced radical population and reduced photoresponse. More direct evidence for structural modification of melanin came from the detection of soluble products with absorbance maxima near 260 nm in supernatants collected after γ-irradiation of cells and cell-free melanin. These products, which include thiobarbituric acid (TBA)-reactive aldehydes, were also generated by Fenton reagent treatment of cells and cell-free melanin. In an assay of melanin integrity based on the metal (Bi(+3)) binding capacity of cells, no detectable loss in binding was detected after γ-irradiation. Our results show that melanin in C. neoformans cells is susceptible to some damage by hydroxyl radical formed in lethal radioactive aqueous environments and serves a protective role in melanized fungi that involves sacrificial breakdown.

Published

2011

26. Cryptococcus neoformans as a Model for Radioimmunotherapy of Infections

Author

Ekaterina Dadachova and Arturo Casadevall

Subjects

Infectious and parasitic diseases, RC109-216

Abstract

There is an obvious and urgent need for novel approaches to treat infectious diseases. The use of monoclonal antibodies in therapy of infectious diseases is now experiencing renewed interest. During the last 5 years radioimmunotherapy (RIT), a modality previously developed only for cancer treatment, has been successfully adapted for the treatment of experimental fungal, bacterial, and viral infections. As our model organism for studying the efficacy, mechanisms, potential toxicity, and radioresistance to RIT, as well as for comparison of RIT with the existing antimicrobial therapies we have chosen the encapsulated yeast Cryptococcus neoformans (CN). The success of RIT approach in laboratory studies provides encouragement for feasibility of therapeutically targeting microbes with labeled antibodies. In addition, the creation of “panantibodies” for RIT which would recognize antigens shared by the whole class of pathogens such as fungi, for example, would facilitate the introduction of RIT into the clinic.

Published

2011

27. Physico-chemical evaluation of rationally designed melanins as novel nature-inspired radioprotectors.

Author

Andrew D Schweitzer, Robertha C Howell, Zewei Jiang, Ruth A Bryan, Gary Gerfen, Chin-Cheng Chen, Dennis Mah, Sean Cahill, Arturo Casadevall, and Ekaterina Dadachova

Subjects

Medicine, Science

Abstract

Melanin, a high-molecular weight pigment that is ubiquitous in nature, protects melanized microorganisms against high doses of ionizing radiation. However, the physics of melanin interaction with ionizing radiation is unknown.We rationally designed melanins from either 5-S-cysteinyl-DOPA, L-cysteine/L-DOPA, or L-DOPA with diverse structures as shown by elemental analysis and HPLC. Sulfur-containing melanins had higher predicted attenuation coefficients than non-sulfur-containing melanins. All synthetic melanins displayed strong electron paramagnetic resonance (2.14.10(18), 7.09.10(18), and 9.05.10(17) spins/g, respectively), with sulfur-containing melanins demonstrating more complex spectra and higher numbers of stable free radicals. There was no change in the quality or quantity of the stable free radicals after high-dose (30,000 cGy), high-energy ((137)Cs, 661.6 keV) irradiation, indicating a high degree of radical stability as well as a robust resistance to the ionizing effects of gamma irradiation. The rationally designed melanins protected mammalian cells against ionizing radiation of different energies.We propose that due to melanin's numerous aromatic oligomers containing multiple pi-electron system, a generated Compton recoil electron gradually loses energy while passing through the pigment, until its energy is sufficiently low that it can be trapped by stable free radicals present in the pigment. Controlled dissipation of high-energy recoil electrons by melanin prevents secondary ionizations and the generation of damaging free radical species.

Published

2009

28. Treating cancer as an infectious disease--viral antigens as novel targets for treatment and potential prevention of tumors of viral etiology.

Author

Xing Guo Wang, Ekaterina Revskaya, Ruth A Bryan, Howard D Strickler, Robert D Burk, Arturo Casadevall, and Ekaterina Dadachova

Subjects

Medicine, Science

Abstract

Nearly 20% of human cancers worldwide have an infectious etiology with the most prominent examples being hepatitis B and C virus-associated hepatocellular carcinoma and human papilloma virus-associated cervical cancer. There is an urgent need to find new approaches to treatment and prevention of virus-associated cancers.Viral antigens have not been previously considered as targets for treatment or prevention of virus-associated cancers. We hypothesized that it was possible to treat experimental HPV16-associated cervical cancer (CC) and Hepatitis B-associated hepatocellular carcinoma (HCC) by targeting viral antigens expressed on cancer cells with radiolabeled antibodies to viral antigens. Treatment of experimental CC and HCC tumors with (188)Re-labeled mAbs to E6 and HBx viral proteins, respectively, resulted in significant and dose-dependent retardation of tumor growth in comparison with untreated mice or mice treated with unlabeled antibodies.This strategy is fundamentally different from the prior uses of radioimmunotherapy in oncology, which targeted tumor-associated human antigens and promises increased specificity and minimal toxicity of treatment. It also raises an exciting possibility to prevent virus-associated cancers in chronically infected patients by eliminating cells infected with oncogenic viruses before they transform into cancer.

Published

2007

29. Ionizing radiation changes the electronic properties of melanin and enhances the growth of melanized fungi.

Author

Ekaterina Dadachova, Ruth A Bryan, Xianchun Huang, Tiffany Moadel, Andrew D Schweitzer, Philip Aisen, Joshua D Nosanchuk, and Arturo Casadevall

Subjects

Medicine, Science

Abstract

BackgroundMelanin pigments are ubiquitous in nature. Melanized microorganisms are often the dominating species in certain extreme environments, such as soils contaminated with radionuclides, suggesting that the presence of melanin is beneficial in their life cycle. We hypothesized that ionizing radiation could change the electronic properties of melanin and might enhance the growth of melanized microorganisms.Methodology/principal findingsIonizing irradiation changed the electron spin resonance (ESR) signal of melanin, consistent with changes in electronic structure. Irradiated melanin manifested a 4-fold increase in its capacity to reduce NADH relative to non-irradiated melanin. HPLC analysis of melanin from fungi grown on different substrates revealed chemical complexity, dependence of melanin composition on the growth substrate and possible influence of melanin composition on its interaction with ionizing radiation. XTT/MTT assays showed increased metabolic activity of melanized C. neoformans cells relative to non-melanized cells, and exposure to ionizing radiation enhanced the electron-transfer properties of melanin in melanized cells. Melanized Wangiella dermatitidis and Cryptococcus neoformans cells exposed to ionizing radiation approximately 500 times higher than background grew significantly faster as indicated by higher CFUs, more dry weight biomass and 3-fold greater incorporation of (14)C-acetate than non-irradiated melanized cells or irradiated albino mutants. In addition, radiation enhanced the growth of melanized Cladosporium sphaerospermum cells under limited nutrients conditions.Conclusions/significanceExposure of melanin to ionizing radiation, and possibly other forms of electromagnetic radiation, changes its electronic properties. Melanized fungal cells manifested increased growth relative to non-melanized cells after exposure to ionizing radiation, raising intriguing questions about a potential role for melanin in energy capture and utilization.

Published

2007

30. Targeted killing of virally infected cells by radiolabeled antibodies to viral proteins.

Author

Ekaterina Dadachova, Mahesh C Patel, Sima Toussi, Christos Apostolidis, Alfred Morgenstern, Martin W Brechbiel, Miroslaw K Gorny, Susan Zolla-Pazner, Arturo Casadevall, and Harris Goldstein

Subjects

Medicine

Abstract

The HIV epidemic is a major threat to health in the developing and western worlds. A modality that targets and kills HIV-1-infected cells could have a major impact on the treatment of acute exposure and the elimination of persistent reservoirs of infected cells. The aim of this proof-of-principle study was to demonstrate the efficacy of a therapeutic strategy of targeting and eliminating HIV-1-infected cells with radiolabeled antibodies specific to viral proteins in vitro and in vivo.Antibodies to HIV-1 envelope glycoproteins gp120 and gp41 labeled with radioisotopes bismuth 213 ((213)Bi) and rhenium 188 ((188)Re) selectively killed chronically HIV-1-infected human T cells and acutely HIV-1-infected human peripheral blood mononuclear cells (hPBMCs) in vitro. Treatment of severe combined immunodeficiency (SCID) mice harboring HIV-1-infected hPBMCs in their spleens with a (213)Bi- or (188)Re-labeled monoclonal antibody (mAb) to gp41 resulted in a 57% injected dose per gram uptake of radiolabeled mAb in the infected spleens and in a greater than 99% elimination of HIV-1-infected cells in a dose-dependent manner. The number of HIV-1-infected thymocytes decreased 2.5-fold in the human thymic implant grafts of SCID mice treated with the (188)Re-labeled antibody to gp41 compared with those treated with the (188)Re-control mAb. The treatment did not cause acute hematologic toxicity in the treated mice.The current study demonstrates the effectiveness of HIV-targeted radioimmunotherapy and may provide a novel treatment option in combination with highly active antiretroviral therapy for the eradication of HIV.

Published

2006

31. Evaluating the Targeting of a Staphylococcus-aureus-Infected Implant with a Radiolabeled Antibody In Vivo

Author

Bruce van Dijk, J. Fred F. Hooning van Duyvenbode, Lisanne de Vor, F. Ruben H. A. Nurmohamed, Marnix G. E. H. Lam, Alex J. Poot, Ruud M. Ramakers, Sofia Koustoulidou, Freek J. Beekman, Jos van Strijp, Suzan H. M. Rooijakkers, Ekaterina Dadachova, H. Charles Vogely, Harrie Weinans, and Bart C. H. van der Wal

Subjects

radiolabeling, theranostics, mice, periprosthetic joint infection, Organic Chemistry, General Medicine, S. aureus, Catalysis, infection, Computer Science Applications, Inorganic Chemistry, antibody, SPECT, radioimmunotherapy, Physical and Theoretical Chemistry, Molecular Biology, biodistribution, Spectroscopy

Abstract

Implant infections caused by Staphylococcus aureus are difficult to treat due to biofilm formation, which complicates surgical and antibiotic treatment. We introduce an alternative approach using monoclonal antibodies (mAbs) targeting S. aureus and provide evidence of the specificity and biodistribution of S.-aureus-targeting antibodies in a mouse implant infection model. The monoclonal antibody 4497-IgG1 targeting wall teichoic acid in S. aureus was labeled with indium-111 using CHX-A”-DTPA as a chelator. Single Photon Emission Computed Tomography/computed tomographyscans were performed at 24, 72 and 120 h after administration of the 111In-4497 mAb in Balb/cAnNCrl mice with a subcutaneous implant that was pre-colonized with S. aureus biofilm. The biodistribution of this labelled antibody over various organs was visualized and quantified using SPECT/CT imaging, and was compared to the uptake at the target tissue with the implanted infection. Uptake of the 111In-4497 mAbs at the infected implant gradually increased from 8.34 %ID/cm3 at 24 h to 9.22 %ID/cm3 at 120 h. Uptake at the heart/blood pool decreased over time from 11.60 to 7.58 %ID/cm3, whereas the uptake in the other organs decreased from 7.26 to less than 4.66 %ID/cm3 at 120 h. The effective half-life of 111In-4497 mAbs was determined to be 59 h. In conclusion, 111In-4497 mAbs were found to specifically detect S. aureus and its biofilm with excellent and prolonged accumulation at the site of the colonized implant. Therefore, it has the potential to serve as a drug delivery system for the diagnostic and bactericidal treatment of biofilm.

Published

2023

32. Characterization of IGF2R Molecular Expression in Canine Osteosarcoma as Part of a Novel Comparative Oncology Approach

Author

Charles Boisclair, Ryan Dickinson, Sabeena Giri, Ekaterina Dadachova, and Valerie MacDonald-Dickinson

Subjects

Inorganic Chemistry, Organic Chemistry, General Medicine, osteosarcoma, canine, IGF2R, radioimmunotherapy, immunohistochemistry, comparative oncology, Physical and Theoretical Chemistry, Molecular Biology, Spectroscopy, Catalysis, Computer Science Applications

Abstract

Progress in prognostic factors, treatments, and outcome for both canine and human osteosarcoma (OS) has been minimal over the last three decades. Surface overexpression of the cation independent mannose-6-phosphate/insulin-like growth factor receptor type 2 (IGF2R) has been proven to occur in human OS cells. Subsequently, radioimmunotherapy (RIT) targeting IGF2R has demonstrated promising preliminary results. The main aims of this study were to investigate the expression of IGF2R in spontaneously occurring canine OS cells using immunohistochemistry (IHC) on archived biopsy samples and to assess its prognostic significance. Thirty-four dogs were included in the study. All cases showed that 80–100% of OS cells stained positive for IGF2R. IGF2R overexpression alone was not shown to have prognostic significance using both visual and quantitative methods of IHC staining intensity. This study has established for the first time the consistent expression of IGF2R in spontaneously occurring canine OS. This comparative oncology approach will allow further investigation into RIT as a novel treatment modality; first in canines and then in humans with OS. In addition, further studies should be performed to assess the true prognostic significance of IGF2R overexpression.

Published

2023

33. 225Ac‐labeled CD33‐targeting antibody reverses resistance to Bcl‐2 inhibitor venetoclax in acute myeloid leukemia models

Author

Dale Ludwig, Wojciech Dawicki, Ravendra Garg, Kevin J. H. Allen, Ekaterina Dadachova, and Eileen M. Geoghegan

Subjects

0301 basic medicine, Cancer Research, medicine.medical_treatment, CD33, Sialic Acid Binding Ig-like Lectin 3, Apoptosis, 225Ac‐lintuzumab, Mice, SCID, chemistry.chemical_compound, Mice, 0302 clinical medicine, Antineoplastic Agents, Immunological, hemic and lymphatic diseases, Tumor Cells, Cultured, Original Research, Cancer Biology, Sulfonamides, Myeloid leukemia, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, Leukemia, Myeloid, Acute, Oncology, Proto-Oncogene Proteins c-bcl-2, 030220 oncology & carcinogenesis, Radioimmunotherapy, Female, medicine.drug, Actinium, Combination therapy, Antineoplastic Agents, acute myeloid leukemia, Antibodies, Monoclonal, Humanized, lcsh:RC254-282, 03 medical and health sciences, medicine, Animals, Humans, Radiology, Nuclear Medicine and imaging, Cell Proliferation, venetoclax, Venetoclax, business.industry, Bcl‐2, Cancer, medicine.disease, Bridged Bicyclo Compounds, Heterocyclic, Xenograft Model Antitumor Assays, 030104 developmental biology, Hypomethylating agent, chemistry, Drug Resistance, Neoplasm, Cytarabine, Cancer research, radioimmunotherapy, business

Abstract

Purpose Despite the availability of new drugs, many patients with acute myeloid leukemia (AML) do not achieve remission and outcomes remain poor. Venetoclax is a promising new therapy approved for use in combination with a hypomethylating agent or with low‐dose cytarabine for the treatment of newly diagnosed older AML patients or those ineligible for intensive chemotherapy. 225Actinium‐lintuzumab (225Ac‐lintuzumab) is a clinical stage radioimmunotherapy targeting CD33 that has shown evidence of single‐agent activity in relapsed/refractory AML. Increased expression of MCL‐1 is a mediator of resistance to venetoclax in cancer. Experimental design Here we investigated the potential for 225Ac‐lintuzumab‐directed DNA damage to suppress MCL‐1 levels as a possible mechanism of reversing resistance to venetoclax in two preclinical in vivo models of AML. Results We demonstrated that 225Ac‐lintuzumab in combination with venetoclax induced a synergistic increase in tumor cell killing compared to treatment with either drug alone in venetoclax‐resistant AML cell lines through both an induction of double‐stranded DNA breaks (DSBs) and depletion of MCL‐1 protein levels. Further, this combination led to significant tumor growth control and prolonged survival benefit in venetoclax‐resistant in vivo AML models. Conclusions There results suggest that the combination of 225Ac‐lintuzumab with venetoclax is a promising therapeutic strategy for the treatment of patients with venetoclax‐resistant AML. Clinical trial of this combination therapy (NCT03867682) is currently ongoing., Long‐term survival of adult patients with acute myeloid leukemia (AML) remains unsatisfactory.We describe the results of a mechanistic and efficacy study combining venetoclax (ABT‐199), a recently approved BCL2 inhibitor, and the clinical stage CD33‐targeting antibody radiolabeled with 225Actinium (225Ac‐lintuzumab) in two venetoclax‐resistant AML models in vitro and in vivo. The study demonstrated dramatic synergy of these two drugs both in vitro and in vivo due to the decrease in BCL‐2 and MCL‐1 levels and induction of double DNA strand breaks. Since both venetoclax and 225Ac‐lintuzumab are already used in patients, we anticipate that rapid translation of this combination approach into the clinic will benefit patients with AML.

Published

2021

34. Transcriptomic and genomic changes associated with radioadaptation in Exophiala dermatitidis

Author

Connor Frank, Zachary Schultzhaus, Mackenzie E. Malo, Jillian Romsdahl, Zheng Wang, and Ekaterina Dadachova

Subjects

Ionizing radiation, Biophysics, Biology, Biochemistry, Genome, Melanin, Transcriptome, 03 medical and health sciences, 0302 clinical medicine, Downregulation and upregulation, Structural Biology, Radioadaptation, Gene expression, Genetics, Gene, 030304 developmental biology, ComputingMethodologies_COMPUTERGRAPHICS, Whole genome sequencing, 0303 health sciences, Fungi, biology.organism_classification, Computer Science Applications, 030220 oncology & carcinogenesis, TP248.13-248.65, Exophiala dermatitidis, Biotechnology, Research Article

Abstract

Graphical abstract, Highlights • Exophiala dermatitidis is a constitutively melanized yeast that is highly resistant to ionizing radiation. • We analyzed the genome and transcriptomes of E. dermatitidis strains adapted to chronic ionizing radiation exposure. • Radioadaptation induces transcriptomic but few genomic changes in E. dermatitidis. • Radioadaptation also results in an altered transcriptomic response to subsequent ionizing radiation exposure. • This regulation involves downregulation of basal metabolic processes and upregulation of translation and DNA repair., Melanized fungi have been isolated from some of the harshest radioactive environments, and their ability to thrive in these locations is in part due to the pigment melanin. Melanin imparts a selective advantage to fungi by providing a physical shield, a chemical shield, and possibly a signaling mechanism. In previous work we demonstrated that protracted exposure of the melanized yeast Exophiala dermatitidis to mixed alpha-, beta-, and gamma-emitting radiation resulted in an adapted strain able to mount a unique response to ionizing radiation in the environment in a melanin-dependent fashion. By exploring the genome and transcriptome of this adapted melanized strain relative to a non-irradiated control we determined the altered response was transcriptomic in nature, as whole genome sequencing revealed limited variation. Transcriptomic analysis indicated that of the adapted isolates analyzed, two lineages existed: one like the naïve, non-adapted strain, and one with a unique transcriptomic signature that exhibited downregulation of metabolic processes, and upregulation of translation-associated genes. Analysis of differential gene expression in the adapted strain showed an overlap in response between the control conditions and reactive oxygen species conditions, whereas exposure to an alpha particle source resulted in a robust downregulation of metabolic processes and upregulation of DNA replication and repair genes, and RNA metabolic processes. This suggest previous exposure to radiation primes the fungus to respond to subsequent exposures in a unique way. By exploring this unique response, we have expanded our knowledge of how melanized fungi interact with and respond to ionizing radiation in their environment.

Published

2020

35. Human monoclonal antibodies against Staphylococcus aureus surface antigens recognize in vitro and in vivo biofilm

Author

Bruce van Dijk, Lisanne de Vor, Kok van Kessel, Jeffrey S Kavanaugh, Carla de Haas, Piet C Aerts, Marco C Viveen, Edwin C Boel, Ad C Fluit, Jakub M Kwiecinski, Gerard C Krijger, Ruud M Ramakers, Freek J Beekman, Ekaterina Dadachova, Marnix GEH Lam, H Charles Vogely, Bart CH van der Wal, Jos AG van Strijp, Alexander R Horswill, Harrie Weinans, and Suzan HM Rooijakkers

Subjects

Staphylococcus aureus, General Immunology and Microbiology, QH301-705.5, General Neuroscience, Science, General Medicine, biochemical phenomena, metabolism, and nutrition, General Biochemistry, Genetics and Molecular Biology, biofilm, Medicine, monoclonal antibodies, Biology (General)

Abstract

Implant-associated Staphylococcus aureus infections are difficult to treat because of biofilm formation. Bacteria in a biofilm are often insensitive to antibiotics and host immunity. Monoclonal antibodies (mAbs) could provide an alternative approach to improve the diagnosis and potential treatment of biofilm-related infections. Here, we show that mAbs targeting common surface components of S. aureus can recognize clinically relevant biofilm types. The mAbs were also shown to bind a collection of clinical isolates derived from different biofilm-associated infections (endocarditis, prosthetic joint, catheter). We identify two groups of antibodies: one group that uniquely binds S. aureus in biofilm state and one that recognizes S. aureus in both biofilm and planktonic state. Furthermore, we show that a mAb recognizing wall teichoic acid (clone 4497) specifically localizes to a subcutaneously implanted pre-colonized catheter in mice. In conclusion, we demonstrate the capacity of several human mAbs to detect S. aureus biofilms in vitro and in vivo.

Published

2022

36. Mechanistic Insights into Synergy between Melanin-Targeting Radioimmunotherapy and Immunotherapy in Experimental Melanoma

Author

Kevin J. H. Allen, Rubin Jiao, Rickles David J, Ekaterina Dadachova, Mackenzie E. Malo, and Connor Frank

Subjects

0301 basic medicine, Male, Immunoconjugates, medicine.medical_treatment, Melanoma, Experimental, lcsh:Chemistry, anti-PD-1 immunotherapy, 0302 clinical medicine, lutetium-177, DBA/2 mice, lcsh:QH301-705.5, Immune Checkpoint Inhibitors, Spectroscopy, Melanoma, General Medicine, Combined Modality Therapy, Computer Science Applications, Tumor Burden, Treatment Outcome, Mice, Inbred DBA, 030220 oncology & carcinogenesis, Radioimmunotherapy, Immunotherapy, Combination therapy, actinium-225, Catalysis, Article, Inorganic Chemistry, 03 medical and health sciences, Cell Line, Tumor, medicine, Animals, Humans, Physical and Theoretical Chemistry, Molecular Biology, Melanins, Tumor microenvironment, business.industry, Organic Chemistry, medicine.disease, Survival Analysis, Immune checkpoint, Blockade, Clinical trial, 030104 developmental biology, lcsh:Biology (General), lcsh:QD1-999, Cancer research, radioimmunotherapy, business

Abstract

Melanoma incidence continues to rise, and while therapeutic approaches for early stage cases are effective, metastatic melanoma continues to be associated with high mortality. Immune checkpoint blockade (ICB) has demonstrated clinical success with approved drugs in cohorts of patients with metastatic melanoma and targeted radionuclide therapy strategies showed promise in several clinical trials against various cancers including metastatic melanoma. This led our group to investigate the combination of these two treatments which could be potentially offered to patients with metastatic melanoma not responsive to ICB alone. Previously, we have demonstrated that a combination of humanized anti-melanin antibody conjugated to 213Bismuth and anti-PD-1 ICB reduced tumor growth and increased survival in the Cloudman S91 murine melanoma DBA/2 mouse model. In the current study, we sought to improve the tumoricidal effect by using the long-lived radionuclides 177Lutetium and 225Actinium. Male Cloudman S91-bearing DBA/2 mice were treated intraperitoneally with PBS (Sham), unlabeled antibody to melanin, anti-PD-1 ICB, 177Lutetium or 225Actinium RIT, or a combination of ICB and RIT. Treatment with anti-PD-1 alone or low-dose 177Lutetium RIT alone resulted in modest tumor reduction, while their combination significantly reduced tumor growth and increased survival, suggesting synergy. 225Actinium RIT, alone or in combination with ICB, showed no therapeutic benefit, suggesting that the two radionuclides with different energetic properties work in distinct ways. We did not detect an increase in tumor-infiltrating T cells in the tumor microenvironment, which suggests the involvement of alternative mechanisms that improve the effect of combination therapy beyond that observed in the single therapies.

Published

2020

37. Structure-function analysis and therapeutic efficacy of antibodies to fungal melanin for melanoma radioimmunotherapy

Author

Kevin J. H. Allen, Ruth A. Bryan, Anthony Bowen, Zewei Jiang, D.J. Rickles, Frank Bruchertseifer, Anjana Ray, Joshua D. Nosanchuk, Ekaterina Dadachova, Rubin Jiao, Arturo Casadevall, Ekaterina Revskaya, Arthie Jeyakumar, G. B. Thornton, Mackenzie E. Malo, Beatriz L. Gómez, and Alfred Morgenstern

Subjects

0301 basic medicine, Skin Neoplasms, medicine.medical_treatment, Interacciones hidrofóbicas, lcsh:Medicine, Comparison antictla, Antibodies, Article, Melanin, 03 medical and health sciences, Mice, Structure-Activity Relationship, 0302 clinical medicine, Neoplasmas, Melanoma murino, In vivo, Cell Line, Tumor, medicine, Structure–activity relationship, Animals, Amino Acid Sequence, lcsh:Science, Melanoma, Melanins, Multidisciplinary, biology, Chemistry, lcsh:R, Immunotherapy, Radioimmunotherapy, medicine.disease, Enfermedades, Therapeutic efficacy, 3. Good health, 030104 developmental biology, Immunoglobulin M, Cell culture, 030220 oncology & carcinogenesis, Immunoglobulin G, Cancer research, biology.protein, Murine Melanoma, Eficacia terapéutica, Hydrophobic interactions, lcsh:Q, Antibody

Abstract

Metastatic melanoma remains difficult to treat despite recent approvals of several new drugs. Recently we reported encouraging results of Phase I clinical trial of radiolabeled with 188Re murine monoclonal IgM 6D2 to melanin in patients with Stage III/IV melanoma. Subsequently we generated a novel murine IgG 8C3 to melanin. IgGs are more amenable to humanization and cGMP (current Good Manufacturing Practice) manufacturing than IgMs. We performed comparative structural analysis of melanin-binding IgM 6D2 and IgG 8C3. The therapeutic efficacy of 213Bi- and 188Re-labeled 8C3 and its comparison with anti-CTLA4 immunotherapy was performed in B16-F10 murine melanoma model. The primary structures of these antibodies revealed significant homology, with the CDRs containing a high percentage of positively charged amino acids. The 8C3 model has a negatively charged binding surface and significant number of aromatic residues in its H3 domain, suggesting that hydrophobic interactions contribute to the antibody-melanin interaction. Radiolabeled IgG 8C3 showed significant therapeutic efficacy in murine melanoma, safety towards healthy melanin-containing tissues and favorable comparison with the anti-CTLA4 antibody. We have demonstrated that antibody binding to melanin relies on both charge and hydrophobic interactions while the in vivo data supports further development of 8C3 IgG as radioimmunotherapy reagent for metastatic melanoma.

Published

2018

38. The Third International Symposium on Fungal Stress – ISFUS

Author

Rocco L. Mancinelli, Ekaterina Dadachova, Gerhard H. Braus, Oded Yarden, Tamás Emri, Christina M. Kelliher, Geoffrey M. Gadd, Natalia Requena, Julia Schumacher, Renata C. Pascon, Florian Bauer, Koon Ho Wong, Thiago Olitta Basso, Alexandra C. Brand, Alexander Idnurm, Alistair J. P. Brown, John E. Hallsworth, Claudia B. L. Campos, Laura Selbmann, David E. Levin, István Pócsi, Drauzio E.N. Rangel, Luis M. Corrochano, Reinhard Fischer, Jan Dijksterhuis, Jesús Aguirre, Radames J. B. Cordero, Deborah Bell-Pedersen, Irina S. Druzhinina, Graeme M. Walker, Anna A. Gorbushina, Gilberto U.L. Braga, Alene Alder-Rangel, Guilherme T.P. Brancini, Martin Kupiec, Michelle Momany, and Mikael Molin

Subjects

0301 basic medicine, Entomopathogenic fungi, Medical mycology, business.industry, Ecology (disciplines), 030106 microbiology, fungi, MICOLOGIA MÉDICA, Environmental ethics, Biology, Article, Microbiology, 03 medical and health sciences, Infectious Diseases, Agriculture, Genetics, business, Ecology, Evolution, Behavior and Systematics

Abstract

Stress is a normal part of life for fungi, which can survive in environments considered inhospitable or hostile for other organisms. Due to the ability of fungi to respond to, survive in, and transform the environment, even under severe stresses, many researchers are exploring the mechanisms that enable fungi to adapt to stress. The International Symposium on Fungal Stress (ISFUS) brings together leading scientists from around the world who research fungal stress. This article discusses presentations given at the third ISFUS, held in Sao Jose dos Campos, Sao Paulo, Brazil in 2019, thereby summarizing the state-of-the-art knowledge on fungal stress, a field that includes microbiology, agriculture, ecology, biotechnology, medicine, and astrobiology.

Published

2020

39. Radioimmunotherapy of Blastomycosis in a Mouse Model With a (1→3)-β-Glucans Targeting Antibody

Author

Bruce van Dijk, Elisabeth Snead, Joshua D. Nosanchuk, Ekaterina Dadachova, Kevin J. H. Allen, and Muath Helal

Subjects

Microbiology (medical), medicine.drug_class, medicine.medical_treatment, mouse model, lcsh:QR1-502, Monoclonal antibody, Microbiology, lcsh:Microbiology, 03 medical and health sciences, Antigen, In vivo, Intensive care, Medicine, 030304 developmental biology, Original Research, 0303 health sciences, biology, 030306 microbiology, business.industry, Blastomyces dermatitidis, 213Bismuth, medicine.disease, biology.organism_classification, Radioimmunotherapy, biology.protein, radioimmunotherapy, (1→3)-β-glucan, Antibody, business, Blastomycosis

Abstract

Invasive fungal infections (IFI) cause devastating morbidity and mortality, especially in organ transplant patients, cancer patients and patients in intensive care units, with the number of IFIs more than tripling since 1979. Radioimmunotherapy (RIT) utilizes antigen-antibody interaction to deliver lethal doses of ionizing radiation to cells and has demonstrated efficacy in several types of cancer. Our laboratories were the first to demonstrate that microorganism-specific monoclonal antibodies are highly effective in treatment of experimental fungal, bacterial and viral infections. Later we proposed to utilize surface expressed antigens shared by major IFI-causing pathogens such as melanin, heat shock protein 60 (HSP60) and beta-glucans as targets for radiolabeled antibodies. Here we evaluated in vivo RIT targeting pan-antigens in IFIs. Blastomycosis dermatitidis was chosen as a model for this work as it causes serious infections in immunocompromised patients, immunocompetent individuals and in companion dogs. B. dermatitidis cells were treated with the 400-2 antibody to (1→3)-β-glucans which was radiolabeled with the beta particles emitter 177Lutetium (177Lu) and alpha particles emitter 213Bismuth (213Bi) and the efficacy of cell kill was determined by CFUs. To determine the antigen-specific localization of the 400-2 antibody in vivo, C57BL6 mice were infected intratracheally with 2×105 B. dermatitidis cells and given 111In-400-2 antibody 24 hr later. To evaluate the killing of B. dermatitidis cells with RIT, intratracheally infected mice were treated with 150 µCi 213Bi-400-2 and their lungs analyzed for CFUs 96 hrs post-infection. 213Bi-400-2 proved to be more effective in killing B. dermatitidis cells in vitro than 177Lu-400-2. Three times more 111In-400-2 accumulated in the lungs of infected mice, than in the non-infected ones. 213Bi-400-2 lowered the fungal burden in the lungs of infected mice more than 2 logs in comparison with non-treated infected controls. In conclusion, our results demonstrate the ability of an anti-(1-3)-beta-D-glucan antibody armed with an alpha-emitter 213Bi to selectively kill B. dermatitidis cells in vitro and in vivo. These results provide strong evidence of the effectiveness of RIT targeting pan-antigens on fungal pathogens.

Published

2020

40. Daratumumab-225Actinium conjugate demonstrates greatly enhanced antitumor activity against experimental multiple myeloma tumors

Author

Kevin J. H. Allen, Mark Berger, Ekaterina Dadachova, Wojciech Dawicki, Dale Ludwig, Rubin Jiao, Muath Helal, and Mackenzie E. Malo

Subjects

0301 basic medicine, lcsh:Immunologic diseases. Allergy, medicine.drug_class, medicine.medical_treatment, Immunology, Monoclonal antibody, lcsh:RC254-282, 03 medical and health sciences, 0302 clinical medicine, immune system diseases, hemic and lymphatic diseases, medicine, Immunology and Allergy, 225actinium, microspect/ct, Multiple myeloma, Antitumor activity, Effector, Chemistry, Daratumumab, medicine.disease, daratumumab, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, multiple myeloma, 030104 developmental biology, Oncology, 030220 oncology & carcinogenesis, Radioimmunotherapy, Cancer research, radioimmunotherapy, lcsh:RC581-607, Conjugate

Abstract

Daratumumab is an anti-CD38 directed monoclonal antibody approved for the treatment of multiple myeloma (MM) and functions primarily via Fc-mediated effector mechanisms such as complement-dependent cytotoxicity (CDC), antibody-dependent cell cytotoxicity (ADCC), antibody-dependent cellular phagocytosis, and T-cell activation. However, not all patients respond to daratumumab therapy and management of MM remains challenging. Radioimmunotherapy with alpha particle-emitting radionuclides represents a promising approach to significantly enhance the potency of therapeutic antibodies in cancer treatment. Here we report the results of mechanistic and feasibility studies using daratumumab radiolabeled with an alpha-emitter 225Actinium for therapy of MM. CD38-positivelymphoma Daudi cell line and MM cell lines KMS-28BM and KMS-28PE were treated in vitro with 225Ac-daratumumab. 225Ac-daratumumab Fc-functional properties were assessed with C1q binding and ADCC assays. The pharmacokinetics and tumor uptake of 111In-daratumumab in Daudi tumor-bearing severe combined immunodeficiency (SCID) mice were measured with microSPECT/CT. The therapeutic effects of 225Ac-daratumumab on Daudi and KSM28BM tumors in mice and treatment side effects were evaluated for 50 days posttreatment. The safety of 225Ac-labeled antimurine CD38 mAb in immunocompetent mice was also evaluated. 225Ac-daratumumab efficiently and specifically killed CD38-positive tumor cells in vitro, while its complement binding and ADCC functions remained unaltered. MicroSPECT/CT imaging demonstrated fast clearance of the radiolabeled daratumumab from the circulation and tissues, but prolonged retention in the tumor up to 10 days. Therapy and safety experiments with 225Ac-daratumumab showed a significant increase in the antitumor potency in comparison to naked antibody without any significant side effects. Our results highlight the potential of targeting alpha-emitters to tumors as a therapeutic approach and suggest that 225Ac-daratumumab may be a promising therapeutic strategy for the treatment of hematologic malignancies.

Published

2019

41. Detection and targeting insulin growth factor receptor type 2 (IGF2R) in osteosarcoma PDX in mouse models and in canine osteosarcoma tumors

Author

Rubin Jiao, Sharayu Karkare, Kevin J. H. Allen, Valerie MacDonald-Dickinson, Mackenzie E. Malo, Bang H. Hoang, Muath Helal, Richard Gorlick, Ekaterina Dadachova, David S. Geller, Ryan M Dickinson, Dale L. Godson, Wojciech Dawicki, and Rui Yang

Subjects

0301 basic medicine, Biodistribution, Immunoconjugates, Single Photon Emission Computed Tomography Computed Tomography, medicine.medical_treatment, lcsh:Medicine, Canine Osteosarcoma, Article, Bone and Bones, Receptor, IGF Type 2, 03 medical and health sciences, Mice, 0302 clinical medicine, Targeted therapies, Dogs, Growth factor receptor, Cell Line, Tumor, Medicine, Animals, Humans, Dog Diseases, lcsh:Science, Cell Proliferation, Osteosarcoma, Multidisciplinary, Molecular medicine, business.industry, Cell growth, lcsh:R, Insulin-like growth factor 2 receptor, X-Ray Microtomography, Radioimmunotherapy, medicine.disease, Xenograft Model Antitumor Assays, 030104 developmental biology, Cancer research, Immunohistochemistry, Feasibility Studies, lcsh:Q, Female, business, 030217 neurology & neurosurgery

Abstract

Osteosarcoma (OS) represents 3.4% of all childhood cancers with overall survival of 70% not improving in 30 years. The consistent surface overexpression of insulin-like growth factor-2 receptor (IGF2R) has been reported in commercial and patient-derived xenograft (PDX) OS cell lines. We aimed to assess efficacy and safety of treating PDX and commercial OS tumors in mice with radiolabeled antibody to IGF2R and to investigate IGF2R expression on canine OS tumors. IGF2R expression on human commercial lines 143B and SaOS2 and PDX lines OS-17, OS-33 and OS-31 was evaluated by FACS. The biodistribution and microSPECT/CT imaging with 111Indium-2G11 mAb was performed in 143B and OS-17 tumor-bearing SCID mice and followed by radioimmunotherapy (RIT) with 177Lutetium-2G11 and safety evaluation. IGF2R expression in randomly selected canine OS tumors was measured by immunohistochemistry. All OS cell lines expressed IGF2R. Biodistribution and microSPECT/CT revealed selective uptake of 2G11 mAb in 143B and OS-17 xenografts. RIT significantly slowed down the growth of OS-17 and 143B tumors without local and systemic toxicity. Canine OS tumors expressed IGF2R. This study demonstrates the feasibility of targeting IGF2R on OS in PDX and spontaneous canine tumors and sets the stage for further development of RIT of OS using comparative oncology.

Published

2019

42. 32-Phosphorus selectively delivered by listeria to pancreatic cancer demonstrates a strong therapeutic effect

Author

Benson Chellakkan Selvanesan, Dinesh Chandra, Ziqiang Yuan, Ekaterina Dadachova, Amanda P. Beck, Steven K. Libutti, Kun Zhu, Arturo Casadevall, Claudia Gravekamp, and Wade Koba

Subjects

0301 basic medicine, Pathology, medicine.medical_specialty, Stromal cell, listeria monocytogenes, Transgene, delivery platform, pancreatic cancer, Panc-02, Endogeny, Antineoplastic Agents, medicine.disease_cause, 32P, 03 medical and health sciences, Mice, 0302 clinical medicine, Immune system, Drug Delivery Systems, Listeria monocytogenes, Pancreatic cancer, medicine, Animals, 2. Zero hunger, Tumor microenvironment, Microscopy, Confocal, biology, business.industry, biology.organism_classification, medicine.disease, 3. Good health, Mice, Inbred C57BL, Pancreatic Neoplasms, KPC, Disease Models, Animal, 030104 developmental biology, Oncology, 030220 oncology & carcinogenesis, Cancer research, Listeria, business, Phosphorus Radioisotopes, Research Paper

Abstract

Our laboratory has developed a novel delivery platform using an attenuated non-toxic and non-pathogenic bacterium Listeria monocytogenes that infects tumor cells and selectively survives and multiplies in metastases and primary tumors with help of myeloid-derived suppressor cells (MDSC) and immune suppression in the tumor microenvironment (TME). 32P was efficiently incorporated into the Listeria bacteria by starvation of the bacteria in saline, and then cultured in phosphorus-free medium complemented with 32P as a nutrient. Listeria-32P kills tumor cells through both 32P-induced ionizing radiation and Listeria-induced reactive oxygen species (ROS). The levels of 32P and Listeria were studied in various normal and tumor tissues, at sequential time points after injection of mice with pancreatic cancer (syngeneic model Panc-02). We found that 32P and Listeria predominantly accumulated in tumors and metastases, with their highest accumulation 4 hrs (32P) and 3 days (Listeria) after injection. Listeria also penetrated the transgenic KPC (conditionally express endogenous Kras-G12D and p53-R172H mutant alleles) pancreatic tumors and metastases. This is remarkable since KPC tumors, like human tumors, exhibit a stromal barrier, which prevents most drugs from penetrating the pancreatic tumors. Therapeutic treatment with Listeria -32P resulted in a strong reduction of the growth of pancreatic cancer at early and late stages in Panc-02 and KPC mice. These results highlight the power of Listeria as new delivery platform of anticancer agents to the TME. Not only were therapeutic levels of radioactive Listeria reached in tumors and metastases but the selective delivery also led to minimal side effects.

Published

2017

43. Reverse Engineering To Characterize Redox Properties: Revealing Melanin's Redox Activity through Mediated Electrochemical Probing

Author

Zülfikar Temoçin, Mijeong Kang, Eunkyoung Kim, Alessandra Napolitano, Lucia Panzella, Jinyang Li, Zheng Wang, William E. Bentley, Gregory F. Payne, Ekaterina Dadachova, Kırıkkale Üniversitesi, Kang, Mijeong, Kim, Eunkyoung, Temocin, Zulftkar, Li, Jinyang, Dadachova, Ekaterina, Wang, Zheng, Panzella, Lucia, Napolitano, Alessandra, Bentley, William E., and Payne, Gregory F.

Subjects

0301 basic medicine, integumentary system, Chemistry, General Chemical Engineering, 02 engineering and technology, General Chemistry, 021001 nanoscience & nanotechnology, Electrochemistry, Redox, Redox Activity, Melanin, 03 medical and health sciences, Electron transfer, 030104 developmental biology, Neuromelanin, Electrode, Materials Chemistry, Biophysics, HUMAN SUBSTANTIA-NIGRA, SHEWANELLA-ALGAE BRY, CRYPTOCOCCUS-NEOFORMANS, ELECTRON-TRANSFER, OXIDATIVE STRESS, FUNGAL MELANINS, ACETAMINOPHEN HEPATOTOXICITY, PHEOMELANIN, EUMELANIN, NEUROMELANIN, 0210 nano-technology, Hydrogel film

Abstract

Temocin, Zulfikar/0000-0001-7151-9772; Panzella, Lucia/0000-0002-2662-8205; Payne, Gregory/0000-0001-6638-9459 WOS: 000444792800003 Melanins are ubiquitous in nature, yet their functions remain poorly understood, because their structures and properties elude characterization by conventional methods. Since many of the proposed functions of melanins (e.g., antioxidant, pro-oxidant, and radical scavenging) involve an exchange of electrons, we developed an electrochemical reverse engineering methodology to probe the redox properties of melanin. This mediated electrochemical probing (MEP) method (i) characterizes insoluble melanin particles that are localized adjacent to an electrode within a permeable hydrogel film, (ii) employs diffusible mediators to shuttle electrons between the electrode and melanin sample, and (iii) imposes complex sequences of input voltages and analyzes output response characteristics (e.g., currents) to reveal redox properties. Here, we illustrate the versatility of MEP and review results demonstrating that melanins have reversible redox activities, can exchange electrons with various reductants and oxidants, and can quench radicals either by donating or accepting electrons. These results suggest possible biological functionalities for melanin and motivate the use of MEP for characterizing additional (i.e., synthesized) materials whose functions rely on redox properties. More broadly, MEP is revealing a richness to redox activities that has previously been inaccessible to investigation. United States National Science FoundationNational Science Foundation (NSF) [DMREF-1435957]; Department of Defense (Defense Threat Reduction Agency)United States Department of DefenseDefense Threat Reduction Agency [HDTRA1-13-1-0037, HDTRA1-15-1-0058] The authors gratefully acknowledge financial support from the United States National Science Foundation (No. DMREF-1435957) and the Department of Defense (Defense Threat Reduction Agency; Nos. HDTRA1-13-1-0037 and HDTRA1-15-1-0058).

Published

2018

44. 627. Differences in C. difficile Toxin A Binding in Humans: Adults vs. Infants

Author

Ahmed Elshazly, Ekaterina Dadachova, Michelle Ewart, and David L. Goldman

Subjects

Abstracts, Infectious Diseases, Text mining, Oncology, B. Poster Abstracts, business.industry, Clostridium difficile toxin A, Medicine, C difficile, business, Microbiology

Abstract

Background Children less than 1 year of age are commonly colonized with toxin-producing C. difficile, but appear to be immune to the associated colitis. Animal studies suggest that young infants lack receptors for C. difficile toxin, though this has never been documented in humans. Methods Tissue from infants ( 21 years were studied. Toxin A binding was assessed using an indirect staining method, which included incubation with toxin A (List Labs) and detection with a rabbit polyclonal anti-sera (Lee Labs). A trained pediatric pathologist assessed the extent of staining in a blinded fashion. In other studies, toxin A was labeled with rhenium-188 and incubated with albumin-blocked tissue sections (four-infant and six-adult) for 1 hour. After washing, gamma counts were measured and the average percentage of retained radiolabeled toxin A calculated. Fisher exact tests and ANOVA were used for analyses. All studies were done in compliance with our institutional IRB. Results Six of 13 (46%) adult specimens were found to have reactivity on both the apical epithelial surface as well as crypt staining. Another six had reactivity localized only to the basal and lateral surface of the crypts. One specimen demonstrated no reactivity at all. For neonates (n = 15), no specimens were found to have reactivity localized to the apical epithelial surface, though four specimens had reactivity at the basal epithelial surface (P value for comparison of apical staining 0.0046) (see figure). Average percentage of retained counts for control (no tissue), infant and adult colon sections were, 0.318 ± 0.147, 0.305 ± 0.079 and 0.48 ± 0.114, respectively (P = 0.051). Conclusion Immunohistochemistry and radiolabelling studies indicate that neonatal colon section binds C. difficile toxin A less strongly and in a different distribution pattern (i.e., without apical staining) when compared with adult colon sections. These findings are consistent with previous animal studies and support the paradigm that a lack of toxin receptors in the infant colon contributes to immunity against C. difficile colitis. Additional studies are needed to define the presence of specific receptors and determine if a similar phenomenon applies to toxin B binding. Disclosures All authors: No reported disclosures.

Published

2018

45. Combined treatment of the experimental human papilloma virus-16-positive cervical and head and neck cancers with cisplatin and radioimmunotherapy targeting viral E6 oncoprotein

Author

Wade Koba, Xing Guo Wang, Arturo Casadevall, Rebecca Phaeton, Zewei Jiang, Ekaterina Dadachova, Matthew Harris, and Gary L. Goldberg

Subjects

Oncology, Cancer Research, medicine.medical_specialty, viruses, medicine.medical_treatment, Transplantation, Heterologous, cisplatin, Mice, Nude, Uterine Cervical Neoplasms, Biology, 03 medical and health sciences, Mice, 0302 clinical medicine, Combined treatment, Internal medicine, medicine, Animals, Humans, Head and neck, Radionuclide Imaging, 030304 developmental biology, Cisplatin, Human papilloma virus, HPV16+cervical cancer, 0303 health sciences, Human papillomavirus 16, HPV16+E6 oncogene, Oncogene Proteins, Viral, Radioimmunotherapy, medicine.disease, Combined Modality Therapy, 3. Good health, Repressor Proteins, HPV16+HNSCC, Head and Neck Neoplasms, 030220 oncology & carcinogenesis, Papilloma, Female, Translational Therapeutics, Neoplasm Transplantation, medicine.drug

Abstract

Background: Human papilloma virus (HPV) is implicated in >99% of cervical cancers and ∼40% of head and neck squamous cell carcinoma (HNSCC). We previously targeted E6 oncogene with 188Rhenium-labelled monoclonal antibody (mAb) C1P5 to HPV16 E6 in cervical cancer and HNSCC. Intranuclear E6 can be accessed by mAbs in non-viable cells with leaky membranes. As radioimmunotherapy (RIT) efficacy depends on the availability of target protein—we hypothesised that pretreatment with cisplatin will kill some tumour cells and increase E6 availability for RIT. Methods Mice with subcutaneous HPV16+ cervical (CasKi) and HNSCC (2A3) tumours were pretreated with 0–7.5 mg kg−1 per day cisplatin for 3 days followed by 188Re-C1P5 and biodistribution was performed 24 h later. For RIT, the animals were treated with: 5 mg kg−1 per day cisplatin for 3 days; or 5 mg kg−1 per day cisplatin for 3 days followed 200 or 400μCi 188Re-C1P5 mAb; or 200 or 400μCi 188Re-C1P5 mAb; or left untreated, and observed for tumour growth for 24 days. Results: Pretreatment with cisplatin increased the uptake of 188Re-C1P5 in the tumours 2.5 to 3.5-fold and caused significant retardation in tumour growth for CasKi and 2A3 tumours in both RIT alone and cisplatin, and RIT groups in comparison with the untreated control and cisplatin alone groups (P

Published

2013

46. Structural Characterization of Melanin Pigments from Commercial Preparations of the Edible Mushroom Auricularia auricula

Author

Ekaterina Dadachova, Ruth E. Stark, Paul Tumpowsky, Arturo Casadevall, Rafael Prados-Rosales, Stacy Toriola, Antonio Nakouzi, Subhasish Chatterjee, and Gary J. Gerfen

Subjects

Indoles, Magnetic Resonance Spectroscopy, Population, Fungus, Naphthols, Article, Cell wall, Melanin, Pigment, Microscopy, Electron, Transmission, Cell Wall, education, Cryptococcus neoformans, Melanins, education.field_of_study, Mushroom, biology, integumentary system, Basidiomycota, Electron Spin Resonance Spectroscopy, General Chemistry, biology.organism_classification, Edible mushroom, Biochemistry, visual_art, visual_art.visual_art_medium, Microscopy, Electron, Scanning, sense organs, Powders, General Agricultural and Biological Sciences

Abstract

Many of the most widely consumed edible mushrooms are pigmented, and these have been associated with some beneficial health effects. Nevertheless, the majority of the reported compounds associated with these desirable properties are non-pigmented. We have previously reported that melanin pigment from the edible mushroom Auricularia auricula can protect mice against ionizing radiation, although no physicochemical characterization was reported. Consequently, in this study we have characterized commercial A. auricula mushroom preparations for melanin content and carried out structural characterization of isolated insoluble melanin materials using a panel of sophisticated spectroscopic and physical/imaging techniques. Our results show that approximately 10% of the dry mass of A. auricula is melanin and that the pigment has physicochemical properties consistent with those of eumelanins, including hosting a stable free radical population. Electron microscopy studies show that melanin is associated with the mushroom cell wall in a manner similar to that of melanin from the model fungus C. neoformans. Elemental analysis of melanin indicated C, H, and N ratios consistent with 5,6-dihydroxyindole-2-carboxylic acid/5,6-dihydroxyindole and 1,8-dihydroxynaphthalene eumelanin. Validation of the identity of the isolated product as melanin was achieved by EPR analysis. A. auricula melanin manifested structural differences, relative to the C. neoformans melanin, with regard to the variable proportions of alkyl chains or oxygenated carbons. Given the necessity for new oral and inexpensive radioprotective materials coupled with the commercial availability of A. auricula mushrooms, this product may represent an excellent source of edible melanin.

Published

2015

47. Fungal stress biology: a preface to the Fungal Stress Responses special edition

Author

Roger D. Finlay, Jan Dijksterhuis, Alene Alder-Rangel, Ekaterina Dadachova, Luis M. Corrochano, John E. Hallsworth, Drauzio E.N. Rangel, Gilberto U.L. Braga, Martin Kupiec, and Universidad de Sevilla. Departamento de Genética

Subjects

Acid, alkali, chaotrope, ethanol, heat, hypoxic, osmotic, and salt stress, Food spoilage, alkali, Adaptation, Biological, osmotic, Context (language use), Saccharomyces cerevisiae, Biology, UV-B radiation tolerance, Bioremediation, Stress, Physiological, Hortaea werneckii, Cryomyces antarcticus, Genetics, Acid, Metarhizium robertsii, Applied research, and salt stress, Beauveria bassiana, Erythritol and mannitol, Food security, Neurospora crassa, business.industry, Ecology, fungi, Compatible solutes, Fungi, food and beverages, Trehalose, chaotrope, General Medicine, hypoxic, Food safety, Astrobiology, Biotechnology, Cochliobolus heterostrophus, Fusarium graminearum, Entomopathogenic fungi, Trichoderma atroviride, Biofuel, Agriculture, Biofuels, ethanol, heat, business, Aspergillus wentii

Abstract

There is currently an urgent need to increase global food security, reverse the trends of increasing cancer rates, protect environmental health, and mitigate climate change. Toward these ends, it is imperative to improve soil health and crop productivity, reduce food spoilage, reduce pesticide usage by increasing the use of biological control, optimize bioremediation of polluted sites, and generate energy from sustainable sources such as biofuels. This review focuses on fungi that can help provide solutions to such problems. We discuss key aspects of fungal stress biology in the context of the papers published in this Special Issue of Current Genetics. This area of biology has relevance to pure and applied research on fungal (and indeed other) systems, including biological control of insect pests, roles of saprotrophic fungi in agriculture and forestry, mycotoxin contamination of the food-supply chain, optimization of microbial fermentations including those used for bioethanol production, plant pathology, the limits of life on Earth, and astrobiology. Brazilian National Council for Scientific and Technological Development (CNPq) 473104/2008-3, 478899/2010-6, PQ2 302312/2011-0, PQ1D 308436/2014-8 São Paulo Research Foundation (FAPESP) of Brazil 2010/06374-1, 2013/50518-6 Ministerio de Educación y Ciencia BIO2012-38520

Published

2015

48. Effects of radiation type and delivery mode on a radioresistant eukaryote Cryptococcus neoformans

Author

Christos Apostolidis, Ekaterina Dadachova, Alfred Morgenstern, Stephen A. Marino, Igor Shuryak, Ruth A. Bryan, and Jack Broitman

Subjects

Cancer Research, Human pathogen, Biology, Radiation Tolerance, Article, Radiolabeled Antibodies, Microbiology, Radiation tolerance, Antibodies monoclonal, Polysaccharides, Radioresistance, Humans, Radiology, Nuclear Medicine and imaging, Cryptococcus neoformans, Cell Nucleus, Cell Death, fungi, Antibodies, Monoclonal, Dose-Response Relationship, Radiation, biology.organism_classification, Delivery mode, Alpha Particles, Gamma Rays, Molecular Medicine, Eukaryote, Bismuth

Abstract

Most research on radioresistant fungi, particularly on human pathogens such as Cryptococcus neoformans, involves sparsely-ionizing radiation. Consequently, fungal responses to densely-ionizing radiation, which can be harnessed to treat life-threatening fungal infections, remain incompletely understood.We addressed this issue by quantifying and comparing the effects of densely-ionizing α-particles (delivered either by external beam or by (213)Bi-labeled monoclonal antibodies), and sparsely-ionizing (137)Cs γ-rays, on Cryptococcus neoformans.The best-fit linear-quadratic parameters for clonogenic survival were the following: α = 0.24 × 10(-2) Gy(-1) for γ-rays and 1.07 × 10(-2) Gy(-1) for external-beam α-particles, and β = 1.44 × 10(-5) Gy(-2) for both radiation types. Fungal cell killing by radiolabeled antibodies was consistent with predictions based on the α-particle dose to the cell nucleus and the linear-quadratic parameters for external-beam α-particles. The estimated RBE (for α-particles vs. γ-rays) at low doses was 4.47 for the initial portion of the α-particle track, and 7.66 for the Bragg peak. Non-radiological antibody effects accounted for up to 23% of cell death.These results quantify the degree of C. neoformans resistance to densely-ionizing radiations, and show how this resistance can be overcome with fungus-specific radiolabeled antibodies.

Published

2015

49. Glycoprotein 41 Targeted Radioimmunotherapy as a Novel Treatment for NeuroHIV/AIDS

Author

Garg, Ravendra, Mills, Kienna, and Ekaterina, Dadachova

Published

2019

50. Microbicidal Power of Alpha Radiation in Sterilizing Germinating Bacillus anthracis Spores

Author

Ekaterina Dadachova, Johanna Rivera, Arturo Casadevall, Alfred Morgenstern, Charles L. Turnbough, Frank Bruchertseifer, and John F. Kearney

Subjects

medicine.drug_class, medicine.medical_treatment, Biology, Monoclonal antibody, Microbiology, Antigen, medicine, Pharmacology (medical), Experimental Therapeutics, Microscopy, Phase-Contrast, Pharmacology, Radioisotopes, Spores, Bacterial, fungi, Antibodies, Monoclonal, biology.organism_classification, Alpha Particles, Bacillus anthracis, Spore, Infectious Diseases, Germination, Radioimmunotherapy, Monoclonal, biology.protein, Antibody, Bismuth

Abstract

Radioimmunotherapy (RIT) takes advantage of the specificity and affinity of the antigen-antibody interaction to deliver microbicidal radioactive nuclides to a site of infection. In this study, we investigated the microbicidal properties of an alpha particle-emitting 213 Bi-labeled monoclonal antibody (MAb), EA2-1 ( 213 Bi-EA2-1), that binds to the immunodominant antigen on Bacillus anthracis spores. Our results showed that dormant spores were resistant to 213 Bi-EA2-1. Significant spore killing was observed following treatment with EA2-1 labeled with 300 μCi 213 Bi; however, this effect was not dependent on the MAb. In contrast, when spores were germinating, 213 Bi-EA2-1 mediated MAb-specific killing in a dose-dependent manner. Dormant spores are very resistant to RIT, and RIT should focus on targeting vegetative cells and germinating spores.

Published

2014