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来自蓝藻聚球藻属菌株PCC7942的番茄红素环化酶的分子结构与酶功能

Molecular structure and enzymatic function of lycopene cyclase from the cyanobacterium Synechococcus sp strain PCC7942.

作者信息

Cunningham F X, Sun Z, Chamovitz D, Hirschberg J, Gantt E

机构信息

Department of Botany, University of Maryland, College Park 20742.

出版信息

Plant Cell. 1994 Aug;6(8):1107-21. doi: 10.1105/tpc.6.8.1107.

Abstract

A gene encoding the enzyme lycopene cyclase in the cyanobacterium Synechococcus sp strain PCC7942 was mapped by genetic complementation, cloned, and sequenced. This gene, which we have named crtL, was expressed in strains of Escherichia coli that were genetically engineered to accumulate the carotenoid precursors lycopene, neurosporene, and zeta-carotene. The crtL gene product converts the acyclic hydrocarbon lycopene into the bicyclic beta-carotene, an essential component of the photosynthetic apparatus in oxygen-evolving organisms and a source of vitamin A in human and animal nutrition. The enzyme also converts neurosporene to the monocyclic beta-zeacarotene but does not cyclize zeta-carotene, indicating that desaturation of the 7-8 or 7'-8' carbon-carbon bond is required for cyclization. The bleaching herbicide 2-(4-methylphenoxy)triethylamine hydrochloride (MPTA) effectively inhibits both cyclization reactions. A mutation that confers resistance to MPTA in Synechococcus sp PCC7942 was identified as a point mutation in the promoter region of crtL. The deduced amino acid sequence of lycopene cyclase specifies a polypeptide of 411 amino acids with a molecular weight of 46,125 and a pI of 6.0. An amino acid sequence motif indicative of FAD utilization is located at the N terminus of the polypeptide. DNA gel blot hybridization analysis indicated a single copy of crtL in Synechococcus sp PCC7942. Other than the FAD binding motif, the predicted amino acid sequence of the cyanobacterial lycopene cyclase bears little resemblance to the two known lycopene cyclase enzymes from nonphotosynthetic bacteria. Preliminary results from DNA gel blot hybridization experiments suggest that, like two earlier genes in the pathway, the Synechococcus gene encoding lycopene cyclase is homologous to plant and algal genes encoding this enzyme.

摘要

通过遗传互补对蓝藻聚球藻属PCC7942菌株中编码番茄红素环化酶的基因进行了定位、克隆和测序。我们将该基因命名为crtL,它在经过基因工程改造以积累类胡萝卜素前体番茄红素、神经孢素和ζ-胡萝卜素的大肠杆菌菌株中表达。crtL基因产物将无环烃番茄红素转化为双环β-胡萝卜素,β-胡萝卜素是放氧生物光合装置的重要组成部分,也是人类和动物营养中维生素A的来源。该酶还将神经孢素转化为单环β-玉米黄质,但不会使ζ-胡萝卜素环化,这表明环化需要7-8或7'-8'碳-碳键的去饱和作用。漂白除草剂2-(4-甲基苯氧基)三乙胺盐酸盐(MPTA)可有效抑制这两种环化反应。在聚球藻属PCC7942中赋予对MPTA抗性的一个突变被鉴定为crtL启动子区域的一个点突变。推导的番茄红素环化酶氨基酸序列确定了一个由411个氨基酸组成的多肽,分子量为46,125,等电点为6.0。一个指示FAD利用的氨基酸序列基序位于多肽的N末端。DNA凝胶印迹杂交分析表明聚球藻属PCC7942中crtL为单拷贝。除了FAD结合基序外,蓝藻番茄红素环化酶的预测氨基酸序列与来自非光合细菌的两种已知番茄红素环化酶几乎没有相似之处。DNA凝胶印迹杂交实验的初步结果表明,与该途径中较早的两个基因一样,聚球藻属编码番茄红素环化酶的基因与植物和藻类中编码该酶的基因同源。

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