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菲咯啉处理的莱茵衣藻y-1中类叶绿素b色素的生物合成

Biosynthesis of a chlorophyllide b-like pigment in phenanthroline-treated Chlamydomonas reinhardtii y-1.

作者信息

Bednarik D P, Hoober J K

出版信息

Arch Biochem Biophys. 1985 Jul;240(1):369-79. doi: 10.1016/0003-9861(85)90042-6.

DOI:10.1016/0003-9861(85)90042-6
PMID:4015109
Abstract

Incubation of degreened Chlamydomonas reinhardtii y-1 cells in the dark with m-phenanthroline induced de novo synthesis of a chlorophyllide b-like pigment. The rate of synthesis of this pigment in the dark was greater than that of total chlorophyll in illuminated cells. Most of the newly synthesized pigment was excreted into the culture medium. The product was extracted from the medium as the metal-free pheophorbide, which had a fluorescence excitation maximum at 428 +/- 1 nm and an emission maximum at 657 +/- 1 nm (E428F657) in ethyl acetate (E427F657 in diethyl ether). Three pheophorbide species were extracted from the medium of green cells treated in the dark, a minor component with a spectrum (E410F670) identical to demetallated chlorophyll a, and two major species with spectral values of E428F657 and E433F657. The latter, predominant form had a spectrum identical to demetallated chlorophyll b, which was purified from the algal cells. E428F657 and E433F657 reacted with hydroxylamine and Girard's T-reagent, which caused a shift in the fluorescence emission maximum to 668 nm. Pheophytin b, which contains an aldehyde group, exhibited an identical spectral shift when treated in the same way, but pheophytin a or porphyrin biosynthetic intermediates did not. Proton NMR analysis of the E428F657 chlorin produced by yellow cells treated with m-phenanthroline confirmed the presence of an aldehydic proton. Chelating and nonchelating phenanthroline analogs equally stimulated synthesis of this product.

摘要

用间菲咯啉在黑暗中培养脱绿的莱茵衣藻y-1细胞,可诱导一种类叶绿素ide b色素的从头合成。该色素在黑暗中的合成速率高于光照细胞中总叶绿素的合成速率。大部分新合成的色素被分泌到培养基中。产物从培养基中提取为无金属的脱镁叶绿酸,其在乙酸乙酯中的荧光激发最大值为428±1 nm,发射最大值为657±1 nm(在乙醚中为E427F657)。从黑暗处理的绿色细胞培养基中提取出三种脱镁叶绿酸,一种次要成分的光谱(E410F670)与脱金属叶绿素a相同,还有两种主要成分的光谱值为E428F657和E433F657。后一种主要形式的光谱与从藻类细胞中纯化得到的脱金属叶绿素b相同。E428F657和E433F657与羟胺和吉拉德T试剂反应,导致荧光发射最大值移至668 nm。含有醛基的脱镁叶绿素b以同样方式处理时表现出相同的光谱位移,但脱镁叶绿素a或卟啉生物合成中间体则没有。用间菲咯啉处理黄色细胞产生的E428F657二氢卟吩的质子核磁共振分析证实了醛基质子的存在。螯合和非螯合的菲咯啉类似物同样刺激该产物的合成。

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