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氨基核苷肾病中肾小球蛋白聚糖的状态

Status of glomerular proteoglycans in aminonucleoside nephrosis.

作者信息

Lelongt B, Makino H, Kanwar Y S

出版信息

Kidney Int. 1987 Jun;31(6):1299-310. doi: 10.1038/ki.1987.143.

Abstract

Status of glomerular proteoglycans (PGs) in puromycin aminonucleoside nephrosis was investigated. Rats were made nephrotic and sacrificed 0, 7, 14, and 21 days later. Maximal proteinuric response was observed between 7 and 14 days. Prior to sacrifice, they received injections of conjugated or unconjugated anti-heparan-sulfate-proteoglycan antibody, directed against its core protein (Mr = 18,000). Their kidneys were processed for direct and indirect immunofluorescence, immunoperoxidase, tannic-acid staining, and tissue autoradiography (ARG). By tannic-acid staining, antibody binding sites identical to the anionic sites described previously were discovered. No qualitative differences were observed by these immunohistochemical techniques. Quantitative tissue ARG did not reveal any statistical differences in the binding of antibody between the control and nephrotic groups. For de novo biosynthetic studies, rats were sacrificed on day 10. Their kidneys were utilized for labeling of basement membrane PGs by employing [35S]-sulfate as the precursor product. Tissue ARG, as well as biochemical studies, were performed on the radiolabeled glomeruli. PGs were extracted with 4 M GuCl and characterized by Sepharose CL-6B and DEAE-Sephacel chromatography. There was an overall increase in the total incorporated radioactivities in the glomerular and media fractions. No differences were observed in the macromolecular size characteristics of intact PGs and glycosaminoglycan chains of either glomerular or media fractions. However, an increase in the charge-density characteristics was observed in PGs of the nephrotic group. By tissue ARG, an increase in the grain densities over the basement membrane and mesangial matrices of the glomerulus was noted. These data indicate that the intact PGs, their chains and core protein do not undergo significant biochemical alterations; however, de novo synthesized PGs have higher charge-density characteristics which may be related to a higher degree of sulfation that occurs during the course of aminonucleoside nephrosis.

摘要

研究了嘌呤霉素氨基核苷肾病中肾小球蛋白聚糖(PGs)的状态。将大鼠制成肾病模型,并在0、7、14和21天后处死。在7至14天之间观察到最大蛋白尿反应。在处死前,它们接受了针对其核心蛋白(Mr = 18,000)的结合或未结合抗硫酸乙酰肝素蛋白聚糖抗体的注射。对它们的肾脏进行直接和间接免疫荧光、免疫过氧化物酶、单宁酸染色和组织放射自显影(ARG)处理。通过单宁酸染色,发现了与先前描述的阴离子位点相同的抗体结合位点。这些免疫组织化学技术未观察到定性差异。定量组织ARG未显示对照组和肾病组之间抗体结合的任何统计学差异。为了进行从头生物合成研究,在第10天处死大鼠。通过使用[35S] - 硫酸盐作为前体产物,将它们的肾脏用于标记基底膜PGs。对放射性标记的肾小球进行组织ARG以及生化研究。用4M胍盐酸盐提取PGs,并通过琼脂糖CL - 6B和DEAE - 琼脂糖凝胶色谱进行表征。肾小球和介质部分中总掺入放射性活性总体增加。在完整PGs以及肾小球或介质部分的糖胺聚糖链的大分子大小特征方面未观察到差异。然而,在肾病组的PGs中观察到电荷密度特征增加。通过组织ARG,注意到肾小球基底膜和系膜基质上的颗粒密度增加。这些数据表明完整的PGs、它们的链和核心蛋白没有发生明显的生化改变;然而,从头合成的PGs具有更高的电荷密度特征,这可能与氨基核苷肾病过程中发生的更高程度的硫酸化有关。

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