AN ULTRASTRUCTURAL STUDY OF GLOMERULAR PERMEABILITY USING CATALASE AND PEROXIDASE AS TRACER PROTEINS

doi:10.1084/jem.132.6.1153

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ARTICLE

AN ULTRASTRUCTURAL STUDY OF GLOMERULAR PERMEABILITY USING CATALASE AND PEROXIDASE AS TRACER PROTEINS

M. A. Venkatachalam M.B., B.S.¹, M. J. Karnovsky M.B., B.Ch.¹, H. D. Fahimi M.D.¹, and R. S. Cotran M.D.¹

¹ From the Harvard Pathology Unit, Mallory Institute of Pathology, Boston City Hospital, Boston, Massachusetts 02118, and the Department of Pathology, Harvard Medical School, Boston, Massachusetts 02115

Mice were injected intravenously with beef liver catalase (molwt 240,000) and very small doses of horseradish peroxidase (molwt 40,000) and the site of localization of these enzymes inthe kidney was studied by ultrastructural cytochemistry. 1 minafter injection, catalase was present in glomerular capillarylumina and there was minimal permeation of the basement membrane.After 5–180 min, staining of the basement membrane increasedprogressively but was usually less than that in capillary lumina.At all time intervals the inner (sub-endothelial) layer of thebasement membrane contained more reaction product than the laminadensa and the outer (subepithelial) layer. Catalase permeatedthe entire thickness of the basement membrane and extended upto the slit pore but not beyond the level of the slit diaphragmand was not seen in the urinary space or tubular lumina. Horseradishperoxidase permeated the whole thickness of the basement membranewithin 2 min after injection; however, gradients of stainingfrom the inner to outer layers of the basement membrane werefrequently seen.

The findings with both enzymes indicate that(a) the basement membrane restricts the passage of proteinsover a wide range of molecular size with increasing impedimentfor larger molecules and (b) the slit pore functions as an additionalbarrier for molecules that cross the basement membrane.

Submitted on July 20, 1970

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