Zhao Xiao-Fan, Wang Jin-Xing, Li Fei-Xue, Sueda Shinji, Kondo Hiroki
Department of Biology, School of Life Sciences, Shandong University, Jinan, 250100, China.
Protein J. 2005 May;24(4):219-25. doi: 10.1007/s10930-005-6714-3.
The cathepsin B-like proteinase from Helicoverpa armigera (HCB) is involved in the degradation of yolk proteins during embryonic development. In order to gain insight into the substrate specificity of this proteinase, various proteins from animals and plants were tested as substrates. The specific cleavage sites of this enzyme on endopeptide bonds were assayed using bovine serum albumin (BSA) as a substrate. Results showed that BSA was degraded into several fragments, which suggests that HCB cleaves BSA at specific endopeptidyl sites. The amino acid sequences of the BSA derived peptides were determined, revealing cleavage of the bonds between residues Arg81-Glu82, Val423-Glu424 and Gly430-Lys431. This suggests that the minimum requirement for a scissile bond to be recognized by HCB is the presence of an ionic amino acid at the P1 ' position and the P1 position can vary. These observations suggest that HCB cleaves bonds at the N-terminal side of ionic amino acid residues giving HCB a wide range of substrates, though other factors dictating the substrate specificity of this enzyme remains to be clarified. Our results provide new evidence that HCB functions as an endopeptidase on some proteins.
棉铃虫的组织蛋白酶B样蛋白酶(HCB)参与胚胎发育过程中卵黄蛋白的降解。为了深入了解这种蛋白酶的底物特异性,对来自动植物的各种蛋白质进行了底物测试。以牛血清白蛋白(BSA)为底物,测定了该酶在内肽键上的特异性切割位点。结果表明,BSA被降解为几个片段,这表明HCB在特定的内肽基位点切割BSA。测定了BSA衍生肽的氨基酸序列,揭示了Arg81-Glu82、Val423-Glu424和Gly430-Lys431残基之间的键被切割。这表明,HCB识别可裂解键的最低要求是在P1'位置存在一个离子氨基酸,且P1位置可以变化。这些观察结果表明,HCB在离子氨基酸残基的N端侧切割键,这使得HCB具有广泛的底物,尽管决定该酶底物特异性的其他因素仍有待阐明。我们的结果提供了新的证据,表明HCB在某些蛋白质上作为一种内肽酶发挥作用。