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在正在生长的棉花子叶细胞间隙中鼠李糖半乳糖醛酸聚糖裂解酶活性的检测与鉴定。

Detection and identification of rhamnogalacturonan lyase activity in intercellular spaces of expanding cotton cotyledons.

作者信息

Naran Radnaa, Pierce Margaret L, Mort Andrew J

机构信息

246 NRC, Department of Biochemistry and Molecular Biology, Oklahoma State University, Stillwater, OK 74078, USA.

出版信息

Plant J. 2007 Apr;50(1):95-107. doi: 10.1111/j.1365-313X.2007.03033.x. Epub 2007 Mar 5.

Abstract

Rhamnogalacturonan lyase (RG lyase) activity has been detected and its relative activity measured in vivo during the expansion of cotton (Gossypium hirsutum L.) cotyledons. Rhamnogalacturonan (RG) oligomers labeled with a fluorescent tag were injected into the intercellular spaces of cotton cotyledons and, after incubation, the digested substrate was rinsed out. Enzyme digestion products were detected and identified by capillary zone electrophoresis. Rhamnogalacturonan lyase products were identified as such by co-migration with the digestion products of linear RG oligomers when the oligomers were treated with fungal RG lyase but not when treated with fungal RG hydrolase. In addition, reaction of plant RG lyase digestion products of RG oligomers with I(2)/KI, which selectively removes unsaturated galactopyranosyluronic acid (GaLap) residues formed at the non-reducing end of the oligomer, converted the plant digestion products into RG oligomers that co-migrated with fungal RG hydrolase products. The activity of the enzyme in the intercellular spaces of cotton cotyledons is very low and could be detected most easily when not >0.03 nmol of substrate was injected in a approximately 0.7-cm(2) area and incubated in vivo for 2-6 h. Rhamnogalacturonan lyase activity was the highest in rapidly expanding 3- to 4-day-old cotyledons and gradually decreased during the slow-down in expansion over the next 2-3 days. The RG lyase activity was also detected when the APTS (8-aminopyrene-1,3,6-trisulfonic acid, trisodium salt)-labeled substrates were introduced into intercellular spaces by infiltration instead of injection, indicating that the activity was not induced by wounding or released into the apoplast by cell damage. An exo-RG galacturonohydrolase activity was also found, but RG hydrolase and exo-RG rhamnohydrolase were not detected.

摘要

在棉花(陆地棉)子叶扩展过程中,已检测到鼠李半乳糖醛酸聚糖裂解酶(RG裂解酶)活性,并在体内测定了其相对活性。将用荧光标签标记的鼠李半乳糖醛酸聚糖(RG)寡聚物注射到棉花子叶的细胞间隙中,孵育后,将消化后的底物冲洗掉。通过毛细管区带电泳检测并鉴定酶消化产物。当用真菌RG裂解酶处理寡聚物时,鼠李半乳糖醛酸聚糖裂解酶产物通过与线性RG寡聚物的消化产物共迁移而被鉴定出来,而用真菌RG水解酶处理时则不然。此外,RG寡聚物的植物RG裂解酶消化产物与I(2)/KI反应,I(2)/KI可选择性去除在寡聚物非还原端形成的不饱和吡喃半乳糖醛酸(GaLap)残基,从而将植物消化产物转化为与真菌RG水解酶产物共迁移的RG寡聚物。棉花子叶细胞间隙中该酶的活性非常低,当在约0.7平方厘米的面积内注射不超过0.03 nmol的底物并在体内孵育2 - 6小时时,最容易检测到。鼠李半乳糖醛酸聚糖裂解酶活性在快速扩展的3至4日龄子叶中最高,并在接下来的2 - 3天扩展减缓过程中逐渐降低。当通过浸润而非注射将APTS(8 - 氨基芘 - 1,3,6 - 三磺酸三钠盐)标记的底物引入细胞间隙时,也检测到了RG裂解酶活性,这表明该活性不是由创伤诱导的,也不是因细胞损伤释放到质外体中的。还发现了一种外切RG半乳糖醛酸水解酶活性,但未检测到RG水解酶和外切RG鼠李糖水解酶。

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