Abstract

Trained, personnel in this core facility will utilize sophisticated state of the art technologies to address and quantitate the physiological significance of the studies proposed in the program project. These important tools include: 1) measurement of force development, 2) determination of monolayer electrical resistance (current impedance), 3) endothelial cell imaging and gap assessment, and 4) quantitation of monolayer permeability. Measurement of force development provides direct quantitation of active tension resulting from activation of the endothelial cell contractile apparatus. Electrical resistance quantitation provides rapid assessment of the opening of conductive gaps (between the borders of adjacent endothelial cells) and focal adhesions (between endothelium and the extracellular matrix. Video imaging of live cells and histologic and confocal imaging of fixed and immunofluorescent-stained cells provides important additional information about the time course, nature, number, and size of paracellular gaps and the overall changes in cell shape. Immunofluorescent imaging furnishes information on the location and organization of key regulatory, contractile, and tethering proteins. Interference reflection microscopy permits quantitation of the changes in focal adhesions between endothelial cells and the matrix. Permeability assessments provides a direct physiological correlate of the critical barrier function that the endothelial cells provide against loss of vascular proteins by quantitation of the rate of albumin transfer across the monolayer grown on a semi-permeable membrane support. Additional services offered by the core are microinjection and measurement of [Ca2+]. Microinjection provides a direct means of altering the intracellular biochemical environment with agents that are not permeable to the plasma membrane, but which are likely to have profound effects on control of contractile and tethering protein assemblies. Ca2+ measurement (based on the fluorescent dye ration method) yields rapid quantitative assessment of one key intracellular signal that controls endothelial barrier function. The tight linkage of these complementary physiologic parameters with the biochemical and molecular results from the various projects will allow assessment of the relative contribution of altered tethering and centripetal forces in producing endothelial cell barrier dysfunction.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Program Projects (P01)
Project #
5P01HL058064-06
Application #
6565062
Study Section
Project Start
2002-02-01
Project End
2003-01-31
Budget Start
Budget End
Support Year
6
Fiscal Year
2002
Total Cost
$197,422
Indirect Cost

  Institution

Name
Johns Hopkins University
Department
Type
DUNS #
045911138
City
Baltimore
State
MD
Country
United States
Zip Code
21218

  Publications

Oita, Radu C; Camp, Sara M; Ma, Wenli et al. (2018) Novel Mechanism for Nicotinamide Phosphoribosyltransferase Inhibition of TNF-?-mediated Apoptosis in Human Lung Endothelial Cells. Am J Respir Cell Mol Biol 59:36-44
Wang, Ting; Brown, Mary E; Kelly, Gabriel T et al. (2018) Myosin light chain kinase ( MYLK) coding polymorphisms modulate human lung endothelial cell barrier responses via altered tyrosine phosphorylation, spatial localization, and lamellipodial protrusions. Pulm Circ 8:2045894018764171
Wang, X; Wang, L; Garcia, J G N et al. (2018) The Significant Role of c-Abl Kinase in Barrier Altering Agonists-mediated Cytoskeletal Biomechanics. Sci Rep 8:1002
Szilágyi, Keely L; Liu, Cong; Zhang, Xu et al. (2017) Epigenetic contribution of the myosin light chain kinase gene to the risk for acute respiratory distress syndrome. Transl Res 180:12-21
Wang, X; Bleher, R; Wang, L et al. (2017) Imatinib Alters Agonists-mediated Cytoskeletal Biomechanics in Lung Endothelium. Sci Rep 7:14152
Shekhawat, Gajendra S; Dudek, Steven M; Dravid, Vinayak P (2017) Development of ultrasound bioprobe for biological imaging. Sci Adv 3:e1701176
Mascarenhas, Joseph B; Tchourbanov, Alex Y; Fan, Hanli et al. (2017) Mechanical Stress and Single Nucleotide Variants Regulate Alternative Splicing of the MYLK Gene. Am J Respir Cell Mol Biol 56:29-37
Belvitch, Patrick; Brown, Mary E; Brinley, Brittany N et al. (2017) The ARP 2/3 complex mediates endothelial barrier function and recovery. Pulm Circ 7:200-210
Camp, Sara M; Chiang, Eddie T; Sun, Chaode et al. (2016) ""Pulmonary Endothelial Cell Barrier Enhancement by Novel FTY720 Analogs: Methoxy-FTY720, Fluoro-FTY720, and ?-Glucuronide-FTY720"". Chem Phys Lipids 194:85-93
Rojo de la Vega, Montserrat; Dodson, Matthew; Gross, Christine et al. (2016) Role of Nrf2 and Autophagy in Acute Lung Injury. Curr Pharmacol Rep 2:91-101

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