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结核分枝杆菌 H37Rv 中氧化应激诱导的 LipD 的分子特征。

Molecular characterization of oxidative stress-inducible LipD of Mycobacterium tuberculosis H37Rv.

出版信息

Curr Microbiol. 2014 Mar;68(3):387-96. doi: 10.1007/s00284-013-0486-3.

DOI:10.1007/s00284-013-0486-3
PMID:24232385
Abstract

The Mycobacterium tuberculosis has developed intricate strategies to evade the killing of microorganism and support its survival in phagocytes. The genome sequence of bacterium revealed the presence of several genes for lypolytic enzymes. Rv1923 gene, a member of Lip family in M. tuberculosis demonstrated the least sequence similarity with its counterpart in non-pathogenic strain M. smegmatis. The expression of Rv1923 gene (LipD) was not observed in in vitro growing cultures of M. tuberculosis H37Ra while an upregulation of transcription of Rv1923 gene was noticed in oxidative conditions. For detailed characterization of LipD enzyme the Rv1923 gene was cloned in pQE30-UA vector and expressed in E. coli M15 cells. LipD was purified from inclusion bodies and refolded with nearly 40 % protein yield. The specific activity of enzyme was calculated to be 16 U/mg with pNP-palmitate as a preferred substrate. Kinetic analysis showed K(m) 0.645 mM and V(max) 24.75 U/ml with pNP-palmitate. Ser-102, Asp-342, and His-369, predicted as the members of the catalytic triad, were confirmed by mutagenesis. Mutagenesis studies revealed that catalytic serine residues located in β-lactamase motifs (S-X-X-K) were responsible for lipolytic activity. Secondary structure analysis by CD spectroscopy demonstrated the presence of α helices and β sheets in the canonical structure of LipD. The enzyme was stable up to 50 °C and was active even at pH 6.0. The expression of enzyme under stress conditions and its activity and stability at high temperature and low pH suggested the possible role of LipD in the survival of mycobacterium in macrophage compartment.

摘要

结核分枝杆菌已经发展出复杂的策略来逃避微生物的杀伤,并支持其在吞噬细胞中的存活。该细菌的基因组序列揭示了几种脂解酶基因的存在。Rv1923 基因是分枝杆菌属 Lip 家族的成员,与非致病性菌株耻垢分枝杆菌的对应物相比,其序列相似性最低。在体外培养的结核分枝杆菌 H37Ra 中观察到 Rv1923 基因(LipD)的表达,但在氧化条件下观察到 Rv1923 基因的转录上调。为了详细表征 LipD 酶,将 Rv1923 基因克隆到 pQE30-UA 载体中,并在大肠杆菌 M15 细胞中表达。从包涵体中纯化 LipD,并通过近 40%的蛋白产率进行复性。该酶的比活性计算为 16 U/mg,以 pNP-棕榈酸为首选底物。动力学分析表明,以 pNP-棕榈酸为底物时,K(m)为 0.645 mM,V(max)为 24.75 U/ml。预测为催化三联体成员的 Ser-102、Asp-342 和 His-369 通过突变得到证实。突变研究表明,位于β-内酰胺酶基序(S-X-X-K)中的催化丝氨酸残基负责脂解活性。圆二色光谱学的二级结构分析表明,LipD 的典型结构中存在α螺旋和β片层。该酶在 50°C 下稳定,甚至在 pH 值为 6.0 时也具有活性。在应激条件下表达酶及其在高温和低 pH 值下的活性和稳定性表明,LipD 可能在分枝杆菌在巨噬细胞区室中的存活中发挥作用。

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