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Increased Production of Zeaxanthin and Other Pigments by Application of Genetic Engineering Techniques to Synechocystis sp. Strain PCC 6803

机译:通过将基因工程技术应用于Synechocystis sp。可以提高玉米黄质和其他色素的产量。应变PCC 6803

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摘要

The psbAII locus was used as an integration platform to overexpress genes involved in carotenoid biosynthesis in Synechocystis sp. strain PCC 6803 under the control of the strong psbAII promoter. The sequences of the genes encoding the yeast isopentenyl diphosphate isomerase (ipi) and the Synechocystis β-carotene hydroxylase (crtR) and the linked Synechocystis genes coding for phytoene desaturase and phytoene synthase (crtP and crtB, respectively) were introduced into Synechocystis, replacing the psbAII coding sequence. Expression of ipi, crtR, and crtP and crtB led to a large increase in the corresponding transcript levels in the mutant strains, showing that the psbAII promoter can be used to drive transcription and to overexpress various genes in Synechocystis. Overexpression of crtP and crtB led to a 50% increase in the myxoxanthophyll and zeaxanthin contents in the mutant strain, whereas the β-carotene and echinenone contents remained unchanged. Overexpression of crtR induced a 2.5-fold increase in zeaxanthin accumulation in the corresponding overexpressing mutant compared to that in the wild-type strain. In this mutant strain, zeaxanthin becomes the major pigment (more than half the total amount of carotenoid) and the β-carotene and echinenone amounts are reduced by a factor of 2. However, overexpression of ipi did not result in a change in the carotenoid content of the mutant. To further alter the carotenoid content of Synechocystis, the crtO gene, encoding β-carotene ketolase, which converts β-carotene to echinenone, was disrupted in the wild type and in the overexpressing strains so that they no longer produced echinenone. In this way, by a combination of overexpression and deletion of particular genes, the carotenoid content of cyanobacteria can be altered significantly.
机译:psbAII基因座被用作整合平台,以过度表达集胞藻属中类胡萝卜素生物合成相关的基因。菌株PCC 6803受强psbAII启动子控制。将编码酵母异戊烯基二磷酸异构酶(ipi)和集胞囊藻β-胡萝卜素羟化酶(crtR)的基因序列以及连接的集胞囊藻去饱和酶和植酮合酶编码的集胞囊藻基因(分别为crtP和crtB)引入到集胞囊藻中psbAII编码序列。 ipi,crtR,crtP和crtB的表达导致突变株中相应的转录水平大量增加,表明psbAII启动子可用于驱动转录并过表达Synechocystis 中的各种基因。 。 crtP crtB 的过表达导致突变菌株中的粘氧叶绿素和玉米黄质含量增加了50%,而β-胡萝卜素和海chin烯酮的含量保持不变。与野生型菌株相比,过量表达 crtR 的玉米黄质在相应的过表达突变体中的积累量增加了2.5倍。在该突变株中,玉米黄质成为主要色素(类胡萝卜素总量的一半以上),β-胡萝卜素和海胆烯酮的量减少了2倍。但是, ipi 的过表达并没有导致突变体的类胡萝卜素含量发生变化。为了进一步改变 Synechocystis 的类胡萝卜素含量,在野生型和野生型中破坏了编码β-胡萝卜素酮醇酶的 crtO 基因,该基因将β-胡萝卜素转化为海胆烯酮。过度表达菌株,以至于它们不再产生produced烯酮。这样,通过特定基因的过度表达和缺失的组合,可以显着改变蓝藻中类胡萝卜素的含量。

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