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Expression and intracellular transport of microvillus membrane hydrolases in human intestinal epithelial cells

机译:微绒毛膜水解酶在人肠上皮细胞中的表达及细胞内转运

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摘要

A panel of monoclonal antibodies was produced against purified microvillus membranes of human small intestinal enterocytes. By means of these probes three disaccharidases (sucrase-isomaltase, lactase- phlorizin hydrolase, and maltase-glucoamylase) and four peptidases (aminopeptidase N, dipeptidylpeptidase IV, angiotension I-converting enzyme, and p-aminobenzoic acid peptide hydrolase) were successfully identified as individual entities by SDS PAGE and localized in the microvillus border of the enterocytes by immunofluorescence microscopy. The antibodies were used to study the expression of small intestinal hydrolases in the colonic adenocarcinoma cell line Caco 2. This cell line was found to express sucrase-isomaltase, lactase-phlorizin hydrolase, aminopeptidase N, and dipeptidylpeptidase IV, but not the other three enzymes. Pulse-chase studies with [35S]methionine and analysis by subunit-specific monoclonal antibodies revealed that sucrase-isomaltase was synthesized and persisted as a single-chain protein comprising both subunits. Similarly, lactase-phlorizin hydrolase was synthesized as a large precursor about twice the size of the lactase subunits found in the human intestine. Aminopeptidase N and dipeptidylpeptidase IV, known to be dimeric enzymes in most mammals, were synthesized as monomers. Transport from the rough endoplasmic reticulum to the trans-Golgi apparatus was considerably faster for the peptidases than for the disaccharidases, as probed by endoglycosidase H sensitivity. These results suggest that the major disaccharidases share a common biosynthetic mechanism that differs from that for peptidases. Furthermore, the data indicate that the transport of microvillus membrane proteins to and through the Golgi apparatus is a selective process that may be mediated by transport receptors.
机译:产生了针对人小肠肠上皮细胞纯化的微绒毛膜的一组单克隆抗体。通过这些探针,成功地鉴定出三个二糖酶(蔗糖酶-异麦芽糖酶,乳糖酶-苯并菲林水解酶和麦芽糖酶-葡糖淀粉酶)和四个肽酶(氨基肽酶N,二肽基肽酶IV,血管紧张素I转化酶和对氨基苯甲酸肽水解酶)。通过SDS PAGE分离单个实体,并通过免疫荧光显微镜检查定位在肠细胞的微绒毛边界。使用该抗体研究结肠腺癌细胞Caco 2中小肠水解酶的表达。发现该细胞表达sucrase-异麦芽糖酶,乳糖酶-phlorizin水解酶,氨肽酶N和二肽基肽酶IV,但不表达其他三种酶。 。用[35S]蛋氨酸进行脉冲追踪研究并通过亚基特异性单克隆抗体进行分析,发现蔗糖酶-异麦芽糖酶已合成并以包含两个亚基的单链蛋白形式存在。相似地,乳糖酶-根皮苷水解酶被合成为一种大的前体,其大小约为人肠中乳糖酶亚基的两倍。氨基肽酶N和二肽基肽酶IV,在大多数哺乳动物中被称为二聚酶,被合成为单体。内切糖苷酶H敏感性表明,肽酶比粗糖质酶从粗糙的内质网向反式高尔基体的转运要快得多。这些结果表明,主要的双糖酶具有与肽酶不同的共同生物合成机制。此外,数据表明,微绒毛膜蛋白向高尔基体的转运和通过高尔基体的转运是一种选择性过程,可能由转运受体介导。

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