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cDNA cloning and primary structure of tryptase from bovine mast cells, and evidence for the expression of bovine pancreatic trypsin inhibitor mRNA in the same cells

机译:牛肥大细胞类胰蛋白酶的cDNA克隆和一级结构,以及牛胰胰蛋白酶抑制剂mRNA在同一细胞中表达的证据

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摘要

A partial cDNA encoding bovine tryptase, an oligomeric serine proteinase previously isolated from bovine mast cells, was obtained by reverse transcription/polymerase chain reaction of mast cell mRNA, using combinations of primers designed on the basis of information obtained from partial sequencing of the purified protein. The complete amino acid sequence of bovine tryptase (245 residues) was deduced from a 711-bp nucleotide sequence and from Edman degradation of the protein. Bovine tryptase primary structure has an identity of about 75% with tryptases from other species and includes all the essential residues of the active-site regions; sequence data in the region of the putative substrate binding pocket suggest a rearrangement capable of maintaining the specificity of trypsin like proteinases. From the same mast cell mRNA, cDNA encoding bovine trypsin protease inhibitor (BPTI) was obtained and amplified with specific primers, confirming the synthesis of BPTI in these cells. Results are consistent with previous data on the presence of BPTI and bovine tryptase in the same granules of bovine mast cells and with their interaction in vitro.
机译:通过使用肥大细胞mRNA的逆转录/聚合酶链反应,并使用根据从纯化蛋白的部分测序获得的信息设计的引物组合,获得了编码牛类胰蛋白酶的部分cDNA,一种先前从牛肥大细胞中分离的寡聚丝氨酸蛋白酶。 。牛类胰蛋白酶的完整氨基酸序列(245个残基)是从711 bp核苷酸序列和蛋白质的埃德曼降解中推导出来的。牛类胰蛋白酶的一级结构与其他物种的类胰蛋白酶具有约75%的同一性,并且包括活性位点区域的所有必需残基;假定的底物结合口袋区域中的序列数据表明能够维持胰蛋白酶样蛋白酶特异性的重排。从相同的肥大细胞mRNA中,获得了编码牛胰蛋白酶蛋白酶抑制剂(BPTI)的cDNA,并用特异性引物进行了扩增,从而证实了这些细胞中BPTI的合成。结果与以前的数据相同,即在相同的牛肥大细胞颗粒中存在BPTI和牛类胰蛋白酶,以及它们在体外的相互作用。

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