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马来酸盐对大鼠肾脏近端小管顶端膜糖蛋白(gp330)的特定作用。

Specific effect of maleate on an apical membrane glycoprotein (gp330) in proximal tubule of rat kidneys.

作者信息

Bergeron M, Mayers P, Brown D

机构信息

Department of Physiology, Université de Montréal, Quebec, Canada.

出版信息

Am J Physiol. 1996 Oct;271(4 Pt 2):F908-16. doi: 10.1152/ajprenal.1996.271.4.F908.

Abstract

Maleate treatment of rats induces transport defects similar to those seen in the Fanconi syndrome (glycosuria, aminoaciduria, phosphaturia, proteinuria, etc.) and causes an accumulation of apical vesicles in proximal tubule epithelial cells. Because the apical membrane glycoprotein, gp330, is a receptor associated with the apical endocytotic and recycling apparatus in these cells, we examined the effect of maleate on the distribution of this protein and other brush border markers. Rats received sodium maleate (400 mg/kg ip) and were killed at various times between 45 min and 3 h; kidneys were perfusion fixed with paraformaldehyde-lysine-periodate before processing for immunofluorescence and immunoelectron microscopy. In control rats, staining with a polyclonal or monoclonal gp330 antibody showed a uniform distribution on the brush border and in coated pits of all proximal tubule cells. In the S3 segments, the immunofluorescence labeling of the microvilli was generally uniform but at times showed spike labeling, suggesting that gp330 sheds easily from the apical membrane. After maleate treatment, the staining intensity of the brush border was decreased in all proximal tubule segments, and cytoplasmic streaks as well as an intense vacuolar staining were seen. In the S3 segment, a remarkable mosaic pattern of staining was observed, with the brush border of some cells being completely negative, while adjacent cells showed an apparently normal staining pattern. These results were confirmed at the electron microscope level, using the protein A-gold technique. Maleate had no effect on the distribution or staining intensity of four other brush border markers, dipeptidyl peptidase IV, and various lectins (Helix pomatia lectin, peanut lectin, elderberry bark lectin). The urinary excretion of gp330 occurs in normal rats and was already increased as early as 1 h after maleate injection and remained at a twofold increment between 6 and 24 h. These data suggest that the generalized membrane transport derangement seen in this experimental Fanconi syndrome could occur via a specific effect on gp330, which seems to block endocytosis and the recycling apparatus at the late endosome level and inhibits the formation of new dense apical tubules.

摘要

用马来酸盐处理大鼠会诱发与范科尼综合征(糖尿、氨基酸尿、磷酸盐尿、蛋白尿等)中所见类似的转运缺陷,并导致近端肾小管上皮细胞顶端小泡的积累。由于顶端膜糖蛋白gp330是与这些细胞顶端内吞和再循环装置相关的一种受体,我们研究了马来酸盐对该蛋白及其他刷状缘标志物分布的影响。给大鼠腹腔注射马来酸钠(400 mg/kg),并在45分钟至3小时之间的不同时间点处死;在进行免疫荧光和免疫电子显微镜检查之前,用多聚甲醛-赖氨酸-高碘酸盐对肾脏进行灌注固定。在对照大鼠中,用多克隆或单克隆gp330抗体染色显示,在所有近端肾小管细胞的刷状缘和被膜小窝中呈均匀分布。在S3段,微绒毛的免疫荧光标记通常是均匀的,但有时会出现棘状标记,提示gp330很容易从顶端膜脱落。马来酸盐处理后,所有近端肾小管段刷状缘的染色强度均降低,可见细胞质条纹以及强烈的空泡染色。在S3段,观察到一种显著的镶嵌染色模式,一些细胞的刷状缘完全阴性,而相邻细胞显示出明显正常的染色模式。使用蛋白A-金技术在电子显微镜水平证实了这些结果。马来酸盐对其他四种刷状缘标志物、二肽基肽酶IV以及各种凝集素(蜗牛凝集素、花生凝集素、接骨木树皮凝集素)的分布或染色强度没有影响。正常大鼠中会出现gp330的尿排泄,早在注射马来酸盐后1小时就已增加,并在6至24小时之间保持两倍的增量。这些数据表明,在这种实验性范科尼综合征中所见的普遍膜转运紊乱可能是通过对gp330的特异性作用而发生的,gp330似乎在晚期内体水平阻断内吞作用和再循环装置,并抑制新的致密顶端小管的形成。

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