首页> 美国卫生研究院文献>Journal of the Boston Society of Medical Sciences >Glomerular anionic site distribution in nonproteinuric rats. A computer-assisted morphometric analysis.
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Glomerular anionic site distribution in nonproteinuric rats. A computer-assisted morphometric analysis.

机译:非蛋白尿大鼠肾小球阴离子位点分布。计算机辅助形态分析。

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摘要

The cationic ultrastructural tracer polyethyleneimine (PEI: pI approximately equal to 11.0), binds electrophysically to uniformly spaced discrete electron-dense anionic sites present in the laminae rarae of the rat glomerular basement membrane (GBM), mesangial reflections of the GBM, Bowman's capsule, and tubular basement membranes when administered intravenously. Computer-assisted morphometric analysis of glomerular anionic sites reveals that the maximum concentration of stainable lamina rara externa (lre) sites (21/10,000 A GBM) occurs 60 minutes after PEI injection with a site-site interspacing of 460 A. Lamina rara interna (lri) sites similarly demonstrate a maximum concentration (20/10,000 A GBM) at 60 minutes with a periodicity of 497 A. The concentration and distribution of anionic sites within the lri was irregular in pattern and markedly decreased in number, while the lre possesses an electrical field that is highly regular at all time intervals analyzed (15, 30, 60, 120, 180, 240, and 300 minutes). Immersion and perfusion of renal tissue with PEI reveals additional heavy staining of the epithelial and endothelial cell sialoprotein coatings. PEI appears to bind to glomerular anionic sites reversibly: ie, between 60 and 180 minutes the concentration of stained sites decreases. At 300 minutes, the interspacing once again approaches the 60-minute concentration. This suggests a dynamic turnover or dissociation followed by a reassociation of glomerular negatively charged PEI binding sites. In contrast, morphometric analysis of anionic sites stained with lysozyme and protamine sulfate reveals interspacings of 642 A and 585 A, respectively; in addition, these tracers produce major glomerular ultrastructural alterations and induce transient proteinuria. PEI does not induce proteinuria in rats, nor does it produce glomerular morphologic alterations when ten times the tracer dosage is administered intravenously. These findings indicate that the choice of ultrastructural charge tracer, the method of administering the tracer, and the time selected for analysis of tissue after administration of tracer significantly influences results. Morphometric analysis of the distribution of glomerular anionic sites in nonproteinuric rats provides a method of evaluating quantitative alterations of the glomerular charge barrier in renal disease models.
机译:阳离子超微结构示踪剂聚乙烯亚胺(PEI:pI大约等于11.0),与大鼠肾小球基底膜(GBM)的层状毛细中均匀分布的电子致密阴离子位点电物理结合,GBM的系膜反射,Bowman胶囊,静脉给药时,以及肾小管基底膜。计算机辅助肾小球阴离子部位的形态计量学分析显示,PEI注射后60分钟出现可染色的椎板外部(lre)部位(21 / 10,000 A GBM)的最大浓度,部位之间的间距为460 A. Iri)位点同样显示60分钟时的最大浓度(20 / 10,000 A GBM),周期性为497A。lri中阴离子位点的浓度和分布呈不规则形式,数量明显减少,而Ire具有在所有分析的时间间隔(15、30、60、120、180、240和300分钟)内高度规则的电场。肾组织浸润和灌注PEI显示上皮和内皮细胞唾液蛋白涂层有额外的重度染色。 PEI似乎可逆地与肾小球阴离子位点结合:即在60到180分钟之间,染色位点的浓度降低。在300分钟时,间隔时间再次接近60分钟的浓度。这表明动态转换或解离,然后肾小球带负电的PEI结合位点重新关联。相反,用溶菌酶和硫酸鱼精蛋白染​​色的阴离子位点的形态分析表明,它们之间的间隔分别为642 A和585A。此外,这些示踪剂产生主要的肾小球超微结构改变,并诱导短暂性蛋白尿。当静脉内施用示踪剂剂量的十倍时,PEI不会在大鼠中诱发蛋白尿,也不会产生肾小球形态改变。这些发现表明,超微结构电荷示踪剂的选择,示踪剂的施用方法以及施用示踪剂后组织分析所选择的时间会显着影响结果。非蛋白尿大鼠肾小球阴离子位点分布的形态计量学分析提供了一种评估肾脏疾病模型中肾小球电荷屏障定量变化的方法。

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