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The crystal structure of the mouse glandular kallikrein-13 (prorenin converting enzyme).

机译:小鼠腺激肽释放酶-13(促肾素原转化酶)的晶体结构。

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摘要

A crystal structure of the serine protease, mouse glandular kallikrein 13 (mGK-13) has been determined at 2.6-A resolution. This enzyme, isolated from the mouse submandibular gland, is also known as prorenin-converting enzyme and cleaves submandibular gland Ren-2 prorenin to yield active renin. The mGK-13 structure is similar to other members of the mammalian serine protease family, having five conserved disulfide bonds and an active site located in the cleft between two beta-barrel domains. The mGK-13 structure reveals for the first time an ordered kallikrein loop conformation containing a short 3(10) helix. This loop is disordered in the related porcine pancreatic kallikrein and rat submandibular tonin structures. The kallikrein loop is in close spatial proximity to the active site and is also involved in a dimeric arrangement of mGK-13. The catalytic specificity of mGK-13 for Ren-2 prorenin was studied by modeling a prorenin-derived peptide into the active site of mGK-13. This model emphasizes two electronegative substrate specificity pockets on the mGK-13 surface, which could accommodate the dibasic P2 and P1 residues at the site of prorenin cleavage by mGK-13.
机译:丝氨酸蛋白酶,小鼠腺激肽释放酶13(mGK-13)的晶体结构已确定在2.6-A分辨率。从小鼠下颌下腺中分离出的这种酶也称为前肾素转化酶,可切割下颌下腺Ren-2肾上腺素以产生活性肾素。 mGK-13结构类似于哺乳动物丝氨酸蛋白酶家族的其他成员,具有五个保守的二硫键和一个位于两个β桶结构域之间的裂缝中的活性位点。 mGK-13结构首次揭示了含有短3(10)螺旋的有序激肽释放酶环构象。该循环在相关的猪胰激肽释放酶和大鼠下颌下单宁结构中紊乱。激肽释放酶环在空间上与活性位点紧密接近,并且也参与mGK-13的二聚体排列。 mGK-13对Ren-2 prorenin的催化特异性是通过将源自prorenin的肽模拟到mGK-13的活性位点来研究的。该模型强调了在mGK-13表面上的两个负电底物特异性口袋,该口袋可容纳mGK-13在肾素原切割位点的二价P2和P1残基。

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