Your search keyword '"Svetlana Krassilnikova"' showing total 2 results

1. Detection of Injury-Induced Vascular Remodeling by Targeting Activated α v β 3 Integrin In Vivo

Author

Amir A. Gharaei, Thomas D. Harris, Jeffrey R. Bender, Ali Kooshkabadi, Hooman Rastegar Fassaei, Scott Edwards, Mehran M. Sadeghi, Leila Esmailzadeh, Jiasheng Zhang, Svetlana Krassilnikova, Albert J. Sinusas, Padmaja Yalamanchili, and Barry L. Zaret

Subjects

Vascular wall, Pathology, medicine.medical_specialty, Apolipoprotein B, Endothelium, Integrin, Arterial Occlusive Diseases, Heterocyclic Compounds, 1-Ring, Mice, Apolipoproteins E, Restenosis, In vivo, Physiology (medical), medicine.artery, Organometallic Compounds, medicine, Animals, Humans, Carotid Stenosis, Common carotid artery, Radioactive Tracers, Cells, Cultured, Cell Proliferation, Mice, Knockout, Tomography, Emission-Computed, Single-Photon, Sulfonamides, biology, Cell growth, business.industry, Carbocyanines, Integrin alphaVbeta3, medicine.disease, medicine.anatomical_structure, biology.protein, Female, Endothelium, Vascular, Cardiology and Cardiovascular Medicine, business

Abstract

Background— The α v β 3 integrin plays a critical role in cell proliferation and migration. We hypothesized that vascular cell proliferation, a hallmark of injury-induced remodeling, can be tracked by targeting α v β 3 integrin expression in vivo. Methods and Results— RP748, a novel 111 In-labeled α v β 3 -specific radiotracer, was evaluated for its cell-binding characteristics and ability to track injury-induced vascular proliferation in vivo. Three groups of experiments were performed. In cultured endothelial cells (ECs), TA145, a cy3-labeled homologue of RP748, localized to α v β 3 at focal contacts. Activation of α v β 3 by Mn 2+ led to increased EC binding of TA145. Left common carotid artery wire injury in apolipoprotein E −/− mice led to vascular wall expansion over a period of 4 weeks. RP748 (7.4 MBq) was injected into groups of 9 mice at 1, 3, or 4 weeks after left carotid injury, and carotids were harvested for autoradiography. Relative autographic intensity, defined as counts/pixel of the injured left carotid area divided by counts/pixel of the uninjured right carotid area, was higher at 1 and 3 weeks (1.8±0.1 and 1.9±0.2, respectively) and decreased significantly by 4 weeks after injury (1.4±0.1, P v and β 3 integrin expression was maximal at 1 week and decreased by 4 weeks after injury. The proliferation index, as determined by Ki67 staining, followed a temporal pattern similar to that of RP748 uptake. Dynamic gamma imaging demonstrated rapid renal clearance of RP748. Conclusions— RP748 has preferential binding to activated α v β 3 integrin and can track the injury-induced vascular proliferative process in vivo.

Published

2004

2. Vascular cell adhesion molecule-1-targeted detection of endothelial activation in human microvasculature

Author

Barry L. Zaret, Svetlana Krassilnikova, N Kirkiles-Smith, Albert J. Sinusas, Amir A. Gharaei, Mehran M. Sadeghi, J.S Schechner, Jeffrey R. Bender, and Jiasheng Zhang

Subjects

Umbilical Veins, Pathology, medicine.medical_specialty, Erythrocytes, Antibody Affinity, Vascular Cell Adhesion Molecule-1, Human skin, Biology, Endothelial activation, Immunoglobulin Fab Fragments, Mice, In vivo, medicine, Animals, Humans, Cell adhesion, Cells, Cultured, Skin, Transplantation, Cell adhesion molecule, Microcirculation, Skin Transplantation, Flow Cytometry, Immunohistochemistry, Molecular biology, Endothelial stem cell, Models, Animal, Surgery, Tumor necrosis factor alpha, Endothelium, Vascular

Abstract

The hallmark of endothelial activation, an early and critical step in many alloimmune and inflammatory responses, is the transcriptional induction and expression of endothelial adhesion molecules (eg, vascular cell adhesion molecule-1 [VCAM-1]). We assessed the feasibility of VCAM-1-targeted in vivo detection of endothelial activation using I-125-labeled-F(ab')2 fragments of E1/6, a monoclonal antibody against human but not murine VCAM-1. The Kd and Bmax, determined by saturation binding in tumor necrosis factor (TNF)-activated human endothelial cells (ECs), were 3.2 +/- 0.6 nmol/L and 5600 +/- 300 binding sites per EC, respectively. Biodistribution and in vivo binding characteristics of I-125-E1/6 F(ab')2 were assessed in a novel chimeric human/mouse model, in which human skin (as a source of human microvasculature) is grafted onto SCID/beige mice. I-125-E1/6 F(ab')2 localized to TNF-activated human skin grafts as detected by autoradiography and gamma well-counting. Relative uptakes (uptake in human skin graft/uptake in the surrounding mouse skin) were, respectively, 2.6 +/- 0.8 (n = 14) and 1.6 +/- 0.3 (n = 12) for E1/6 and MOPC-21, an isotype-matched control antibody (P < .01). The preferential uptake in human skin graft was not due to differences in tissue vascularity assessed by Tc-99m-labeled murine red blood cells. In conclusion, the chimeric human/mouse model is a novel experimental tool for in vivo evaluation of human endothelial cell-specific radiopharmaceuticals. Although I-125-E1/6 F(ab')2 localized to human skin grafts, the limited number of VCAM-1 molecules/endothelial cell adversely affects its suitability as a target for in vivo imaging of endothelial activation.

Published

2004