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Characteristics of an R-Phycoerythrin with Two γ Subunits Prepared from Red Macroalga Polysiphonia urceolata

机译:红色Macroalga polysiphonia urceolata制备的带有两个γ亚基的R-藻红蛋白的特性

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摘要

An R-phycoerythrin (R-PE) was isolated by gel filtrations on Sepharose CL-4B and Sephadex G-150 from the phycobiliprotein extract of the marine red macroalga Polysiphonia urceolata Grev and further purified by ion exchange chromatography on DEAE-Sepharose Fast Flow. The purified R-PE showed three absorption peaks at 498 nm, 538 nm, 566 nm and one fluorescent emission maximum at 577 nm. Although the R-PE showed a single band on the examination by native PAGE, it exhibited two very close bands at pH about 4.7 in native isoelectric focusing (IEF). Polypeptide analysis of the R-PE demonstrated that it contained four chromophore-carrying subunits, α18.2, β20.6, γ31.6 (γ'), γ34.6 (γ), and no colorless polypeptide; its subunit composition was 6α18.2:6β20.6:1 γ31.6:2γ34.6. The α and β subunits were distributed within a acidic pH range from 5.0 to 6.0 in denaturing IEF and the γ subunits were in a basic pH range from 7.6 to 8.1. These results reveal that the prepared R-PE may exist in two hexamers of γ (αβ)3 γ (αβ)3γ' and γ (αβ)3 γ'(αβ)3 γ and that the R-PE participate in the rod domain assembly of P. urceolata phycobilisomes by stacking each of its trimer (αβ)3 face-to-face with the aid of one γ subunit (γ or γ').
机译:通过琼脂糖凝胶CL-4B和Sephadex G-150凝胶过滤从海洋红巨藻Polysiphonia urceolata Grev的藻胆蛋白提取物中分离R-藻红蛋白(R-PE),并在DEAE-Sepharose Fast Flow上通过离子交换色谱进一步纯化。纯化的R-PE在498 nm,538 nm,566 nm处显示三个吸收峰,在577 nm处显示一个最大的荧光发射。尽管R-PE在通过天然PAGE检查时显示一条条带,但在天然等电聚焦(IEF)中,在pH约为4.7时,R-PE表现出两条非常接近的条带。 R-PE的多肽分析表明,它含有四个发色团亚基,α 18.2 ,β 20.6 ,γ 31.6 (γ') ,γ 34.6 (γ),且无色多肽;其亚基组成为6α 18.2 :6β 20.6 :1γ 31.6 :2γ 34.6 。在变性IEF中,α和β亚基分布在5.0到6.0的酸性pH范围内,而γ亚基分布在7.6到8.1的碱性pH范围内。这些结果表明,制备的R-PE可能存在于γ(αβ)3γ(αβ)3γ'和γ(αβ)3γ'(αβ)3γ的两种六聚体中,并且R-PE参与了杆域借助于一个γ亚基(γ或γ')将每个三聚体(αβ)3面对面堆叠起来,从而组装成P. urceolata藻胆体。

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