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Differential expression of two basement membrane collagen genes, COL4A6 and COL4A5, demonstrated by immunofluorescence staining using peptide- specific monoclonal antibodies

机译:使用肽特异性单克隆抗体通过免疫荧光染色证明了两个基底膜胶原蛋白基因COL4A6和COL4A5的差异表达

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摘要

Genes for the human alpha 5(IV) and alpha 6(IV) collagen chains have a unique arrangement in that they are colocalized on chromosome Xq22 in a head-to-head fashion and appear to share a common bidirectional promoter. In addition we reported a novel observation that the COL4A6 gene is transcribed from two alternative promoters in a tissue-specific manner (Sugimoto, M., T. Oohashi, and Y. Ninomiya. 1994. Proc. Natl. Acad. Sci. USA. 91:11679-11683). To know whether the translation products of both genes are colocalized in various tissues, we raised alpha 5(IV) and alpha 6(IV) chain-specific rat monoclonal antibodies against synthetic peptides reflecting sequences near the carboxy terminus of each noncollagenous (NC)1 domain. By Western blotting alpha 6(IV) chain-specific antibody recognized 27-kD monomers and associated dimers of the human type IV collagen NC1 domain, which is the first demonstration of the presence in tissues of the alpha 6(IV) polypeptide as predicted from its cDNA sequence. Immunofluorescence studies using anti-alpha 6(IV) antibody demonstrated that in human adult kidney the alpha 6(IV) chain was never detected in the glomerular basement membrane, whereas the basement membranes of the Bowman's capsules and distal tubules were positive. The staining pattern of the glomerular basement membrane was quite different from that obtained with the anti- alpha 5(IV) peptide antibody. The alpha 5(IV) and alpha 6(IV) chains were colocalized in the basement membrane in the skin, smooth muscle cells, and adipocytes; however, little if any reaction was seen in basement membranes of cardiac muscles and hepatic sinusoidal endothelial cells. Thus, both genes are expressed in a tissue-specific manner, perhaps due to the unique function of the bidirectional promoter for both genes, which is presumably different from that for COL4A1 and COL4A2.
机译:人类alpha 5(IV)和alpha 6(IV)胶原蛋白链的基因具有独特的排列方式,因为它们以头对头的方式共定位在Xq22染色体上,并且似乎共享一个共同的双向启动子。此外,我们报道了一种新颖的观察结果,即以组织特异性方式从两个替代启动子转录了COL4A6基因(Sugimoto,M.,T. Oohashi和Y. Ninomiya。1994. Proc.Natl.Acad.Sci.USA。 91:11679-11683)。为了知道这两个基因的翻译产物是否在各种组织中共定位,我们提出了针对合成肽的α5(IV)和α6(IV)链特异性大鼠单克隆抗体,该单克隆抗体反映了每个非胶原(NC)1羧基末端附近的序列。域。通过蛋白质印迹法,α6(IV)链特异性抗体识别了人类IV型胶原蛋白NC1域的27-kD单体和相关的二聚体,这是从组织中预测的α6(IV)多肽在组织中的首次存在它的cDNA序列。使用抗α6(IV)抗体的免疫荧光研究表明,在成年肾脏中,从未在肾小球基底膜中检测到α6(IV)链,而鲍曼氏囊和远端小管的基底膜是阳性的。肾小球基底膜的染色模式与用抗α5(IV)肽抗体获得的染色模式完全不同。 alpha 5(IV)和alpha 6(IV)链共定位在皮肤,平滑肌细胞和脂肪细胞的基底膜中;但是,在心肌和肝窦窦内皮细胞的基底膜中几乎看不到任何反应。因此,两个基因都以组织特异性方式表达,这可能是由于双向启动子对两个基因的独特功能所致,这可能与COL4A1和COL4A2的功能不同。

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