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Effects of Modified Phycobilin Biosynthesis in the Cyanobacterium Synechococcus sp. Strain PCC 7002

机译:修改后的藻蓝素生物合成对蓝藻Syechococcus sp。的影响。应变PCC 7002

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摘要

The pathway for phycocyanobilin biosynthesis in Synechococcus sp. strain PCC 7002 comprises two enzymes: heme oxygenase and phycocyanobilin synthase (PcyA). The phycobilin content of cells can be modified by overexpressing genes encoding alternative enzymes for biliverdin reduction. Overexpression of the pebAB and HY2 genes, encoding alternative ferredoxin-dependent biliverdin reductases, caused unique effects due to the overproduction of phycoerythrobilin and phytochromobilin, respectively. Colonies overexpressing pebAB became reddish brown and visually resembled strains that naturally produce phycoerythrin. This was almost exclusively due to the replacement of phycocyanobilin by phycoerythrobilin on the phycocyanin α-subunit. This phenotype was unstable, and such strains rapidly reverted to the wild-type appearance, presumably due to strong selective pressure to inactivate pebAB expression. Overproduction of phytochromobilin, synthesized by the Arabidopsis thaliana HY2 product, was tolerated much better. Cells overexpressing HY2 were only slightly less pigmented and blue-green than the wild type. Although the pcyA gene could not be inactivated in the wild type, pcyA was easily inactivated when cells expressed HY2. These results indicate that phytochromobilin can functionally substitute for phycocyanobilin in Synechococcus sp. strain PCC 7002. Although functional phycobilisomes were assembled in this strain, the overall phycobiliprotein content of cells was lower, the efficiency of energy transfer by these phycobilisomes was lower than for wild-type phycobilisomes, and the absorption cross-section of the cells was reduced relative to that of the wild type because of an increased spectral overlap of the modified phycobiliproteins with chlorophyll a. As a result, the strain producing phycobiliproteins carrying phytochromobilin grew much more slowly at low light intensity.
机译:Synechococcus sp。中藻蓝蛋白的生物合成途径。 PCC 7002菌株包含两种酶:血红素加氧酶和藻蓝蛋白合酶(PcyA)。细胞的藻胆素含量可以通过过表达编码biliverdin降低的替代酶的基因来修饰。编码替代铁氧还蛋白依赖的胆绿素还原酶的pebAB和HY2基因的过表达,分别由于藻红蛋白和植物钙转运蛋白的过量生产而引起独特的作用。过表达pebAB的菌落变成红棕色,外观上类似于天然产生藻红蛋白的菌株。这几乎完全是由于藻蓝蛋白α-亚基上的藻红蛋白替代了藻蓝蛋白。该表型是不稳定的,并且这些菌株迅速恢复为野生型外观,大概是由于使pebAB表达失活的强大选择性压力所致。拟南芥HY2产品合成的植物卟啉的生产过剩的耐受性要好得多。过表达HY2的细胞的色素沉着和蓝绿色仅比野生型少。尽管pcyA基因不能在野生型中失活,但是当细胞表达HY2时pcyA容易失活。这些结果表明,藻蓝蛋白可以在功能上替代Synechococcus sp中的藻蓝蛋白。菌株PCC7002。尽管在该菌株中组装了功能性藻胆体,但细胞的总体藻胆蛋白含量较低,这些藻胆体的能量转移效率比野生型藻胆体低,并且细胞的吸收截面减小相对于野生型,因为修饰的藻胆蛋白与叶绿素a的光谱重叠增加。结果,产生携带藻动蛋白的藻胆蛋白的菌株在低光强度下生长得慢得多。

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