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假单胞菌属LDC-25的phaC1/phaC2基因的序列分析、结构预测及功能验证及其在聚羟基脂肪酸酯积累中的重要性。

Sequence analysis, structure prediction, and functional validation of phaC1/phaC2 genes of Pseudomonas sp. LDC-25 and its importance in polyhydroxyalkanoate accumulation.

作者信息

Sujatha Kabilan, Mahalakshmi Ayyasamy, Solaiman Daniel K Y, Shenbagarathai Rajaiah

机构信息

PG Department of Zoology and Biotechnology, Lady Doak College, Madurai - 625 002, Tamilnadu, India.

出版信息

J Biomol Struct Dyn. 2009 Jun;26(6):771-9. doi: 10.1080/07391102.2009.10507289.

Abstract

Polyhydroxyalkanoates (PHAs) are attractive biomaterials in both conventional medical devices and tissue engineering. PHA synthase is responsible for catalyzing the formation of Polyhydroxyalkanoates (PHA), but its structural information is limited. Hence, this study focuses to predict 3D model for phaC1 and phaC2 genes of field-soil strain Pseudomonas sp. LDC-25 and to validate the functional properties through in vitro studies. The phaC1/phaC2 genes were amplified, cloned, and sequenced. The sequence analysis showed > 90% homology to phaC loci and presence of alpha/beta hydrolase fold, but phaC2 loci of LDC-25 exhibits variation in the conserved residue (Ser is replaced by Ala). Threading approach demonstrated that Carboxylesterase (d1tqha) can be used as the modeling template. The predicted models showed the presence of conserved residues at 122 (G), 205 (S), and 236 (S). In vitro studies also supported that PHA accumulation ability was less in Pseudomonas sp. LDC-25 compared to other field isolate, Pseudomonas sp. LDC-5. FT-IR spectrum showed PHA specific peaks at 1735.62 cm(-1). Results of this study would help to detect the functional domains of the protein in order to elucidate their structure/function characteristics with special emphasis on invariant conserved residues.

摘要

聚羟基脂肪酸酯(PHA)在传统医疗器械和组织工程领域都是具有吸引力的生物材料。PHA合酶负责催化聚羟基脂肪酸酯(PHA)的形成,但其结构信息有限。因此,本研究着重预测田间土壤菌株假单胞菌属LDC - 25的phaC1和phaC2基因的三维模型,并通过体外研究验证其功能特性。phaC1/phaC2基因被扩增、克隆并测序。序列分析表明,其与phaC基因座的同源性大于90%,且存在α/β水解酶折叠结构,但LDC - 25的phaC2基因座在保守残基处存在变异(丝氨酸被丙氨酸取代)。穿线法表明羧酸酯酶(d1tqha)可作为建模模板。预测模型显示在122位(甘氨酸)、205位(丝氨酸)和236位(丝氨酸)存在保守残基。体外研究还表明,与其他田间分离株假单胞菌属LDC - 5相比,假单胞菌属LDC - 25的PHA积累能力较低。傅里叶变换红外光谱在1735.62 cm⁻¹处显示出PHA的特定峰。本研究结果将有助于检测该蛋白质的功能域,从而阐明其结构/功能特征,特别关注不变的保守残基。

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