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大肠杆菌生物降解性苏氨酸脱水酶的共价结构:与其他脱水酶的同源性

Covalent structure of biodegradative threonine dehydratase of Escherichia coli: homology with other dehydratases.

作者信息

Datta P, Goss T J, Omnaas J R, Patil R V

出版信息

Proc Natl Acad Sci U S A. 1987 Jan;84(2):393-7. doi: 10.1073/pnas.84.2.393.

Abstract

The 987-base-pair coding region of the tdc gene of Escherichia coli K-12 encoding biodegradative threonine dehydratase [Tdc; L-threonine hydro-lyase (deaminating), EC 4.2.1.16], previously cloned in this laboratory, was sequenced. The deduced polypeptide consists of 329 amino acid residues with a calculated Mr of 35,238. Although the purified enzyme was shown to contain tryptophan, no tryptophan codon was found in the tdc reading frame. Incubation of purified Tdc with [14C]tryptophan revealed apparent "covalent" binding of tryptophan, indicating posttranslational modification of the enzyme. A heptapeptide, 54Thr-55Gly-56Ser-57Phe-58Lys-59Ile- 60Arg, was found to contain Lys-58, which binds pyridoxal phosphate coenzyme. A comparison of amino acid sequences between the Tdc polypeptide and the biosynthetic threonine dehydratases of yeast (encoded by ILV1) and E. coli (encoded by ilvA) and the E. coli D-serine dehydratase (DsdA, encoded by dsdA) revealed various extents of homology: five domains of the Tdc polypeptide were 63-93% homologous with the yeast enzyme, and three of these same regions were 80% homologous with the biosynthetic E. coli dehydratase; two different domains showed 67% and 83% homology with DsdA. In addition, two other sequences were highly conserved in all four proteins, one of which was shown to contain the conserved lysine residue that binds pyridoxal phosphate in the Tdc and DsdA polypeptides. These observations suggest that, despite their diverse origin and metabolic significance, these enzymes may have evolved from a common ancestral protein.

摘要

先前在本实验室克隆的大肠杆菌K-12的tdc基因的987个碱基对编码区,编码生物降解性苏氨酸脱水酶[Tdc;L-苏氨酸水解酶(脱氨基),EC 4.2.1.16],已进行测序。推导的多肽由329个氨基酸残基组成,计算的分子量为35238。尽管纯化的酶显示含有色氨酸,但在tdc阅读框中未发现色氨酸密码子。用[14C]色氨酸孵育纯化的Tdc显示出色氨酸的明显“共价”结合,表明该酶存在翻译后修饰。发现一个七肽,54Thr-55Gly-56Ser-57Phe-58Lys-59Ile-60Arg,含有结合磷酸吡哆醛辅酶的Lys-58。对Tdc多肽与酵母(由ILV1编码)和大肠杆菌(由ilvA编码)的生物合成苏氨酸脱水酶以及大肠杆菌D-丝氨酸脱水酶(DsdA,由dsdA编码)的氨基酸序列进行比较,发现了不同程度的同源性:Tdc多肽的五个结构域与酵母酶的同源性为63-93%,其中相同的三个区域与大肠杆菌生物合成脱水酶的同源性为80%;两个不同的结构域与DsdA显示出67%和83%的同源性。此外,在所有四种蛋白质中,另外两个序列高度保守,其中一个被证明含有在Tdc和DsdA多肽中结合磷酸吡哆醛的保守赖氨酸残基。这些观察结果表明,尽管这些酶起源不同且具有不同的代谢意义,但它们可能是由一个共同的祖先蛋白质进化而来的。

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