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鳞翅目夜蛾科昆虫中肠海藻糖酶活性所必需的催化及其他残基。

The catalytic and other residues essential for the activity of the midgut trehalase from Spodoptera frugiperda.

机构信息

Departamento de Bioquímica, Instituto de Química, Universidade de São Paulo, C.P. 26077, 05513-970 São Paulo, Brazil.

出版信息

Insect Biochem Mol Biol. 2010 Oct;40(10):733-41. doi: 10.1016/j.ibmb.2010.07.006. Epub 2010 Aug 5.

Abstract

Trehalase (EC 3.2.1.28) hydrolyzes only α, α'- trehalose and is present in a variety of organisms, but is most important in insects and fungi. Crystallographic data showed that bacterial trehalase has D312 and E496 as the catalytical residues and three Arg residues in the active site. Those residues have homologous in all family 37 trehalases including Spodoptera frugiperda trehalase (D322, E520, R169, R227, R287). To test the role of these residues, mutants of trehalase were produced. All mutants were at least four orders of magnitude less active than wild type trehalase and no structural difference between these mutants and wild type enzyme were discernible by circular dichroism. D322A and E520 pH-activity profile lacked the alkaline arm and the acid arm, respectively, suggesting that D322 is the acid and E520 the basic catalyst. Azide increases E520A activity three times, confirming its action as the basic catalyst. Taking into account the decrease in activity after substitution for alanine residue, the three arginine residues are as important as the catalytical ones to trehalase activity. This clarifies the previous misidentification of an Arg residue as the acid catalyst. As far as we know, this is the first report on the functional identification residues important for trehalase activity.

摘要

海藻糖酶(EC 3.2.1.28)仅水解α,α'-海藻糖,存在于多种生物体中,但在昆虫和真菌中最为重要。晶体学数据表明,细菌海藻糖酶具有 D312 和 E496 作为催化残基,以及活性位点的三个 Arg 残基。这些残基在所有家族 37 海藻糖酶中都具有同源性,包括草地贪夜蛾海藻糖酶(D322、E520、R169、R227、R287)。为了测试这些残基的作用,产生了海藻糖酶的突变体。所有突变体的活性至少比野生型海藻糖酶低四个数量级,并且这些突变体与野生型酶之间的结构差异通过圆二色性无法辨别。D322A 和 E520 的 pH 活性曲线分别缺乏碱性臂和酸性臂,表明 D322 是酸性催化剂,E520 是碱性催化剂。叠氮化物使 E520A 的活性增加了三倍,证实了它作为碱性催化剂的作用。考虑到用丙氨酸残基取代后活性的降低,三个精氨酸残基对海藻糖酶活性的重要性与催化残基一样重要。这澄清了先前将一个 Arg 残基错误鉴定为酸性催化剂的情况。据我们所知,这是首次报道对海藻糖酶活性重要的功能鉴定残基。

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