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抗坏血酸诱导的羟基自由基对植物细胞壁多糖的氧化裂解

Oxidative scission of plant cell wall polysaccharides by ascorbate-induced hydroxyl radicals.

作者信息

Fry S C

机构信息

The Edinburgh Cell Wall Group, Institute of Cell and Molecular Biology, The University of Edinburgh, The King's Buildings, Edinburgh EH9 3JH, UK.

出版信息

Biochem J. 1998 Jun 1;332 ( Pt 2)(Pt 2):507-15. doi: 10.1042/bj3320507.

Abstract

Scission of plant cell wall polysaccharides in vivo has generally been assumed to be enzymic. However, in the presence of l-ascorbate, such polysaccharides are shown to undergo non-enzymic scission under physiologically relevant conditions. Scission of xyloglucan by 1 mM ascorbate had a pH optimum of 4.5, and the maximum scission rate was reached after a 10-25-min delay. Catalase prevented the scission, whereas added H2O2 (0.1-10 mM) increased the scission rate and shortened the delay. Ascorbate caused detectable xyloglucan scission above approx. 5 microM. Dehydroascorbate was much less effective. Added Cu2+ (>0.3 microM) also increased the rate of ascorbate-induced scission; EDTA was inhibitory. The rate of scission in the absence of added metals appeared to be attributable to the traces of Cu (2.8 mg.kg-1) present in the xyloglucan. Ascorbate-induced scission of xyloglucan was inhibited by radical scavengers; their effectiveness was proportional to their rate constants for reaction with hydroxyl radicals (.OH). It is proposed that ascorbate non-enzymically reduces O2 to H2O2, and Cu2+ to Cu+, and that H2O2 and Cu+ react to form .OH, which causes oxidative scission of polysaccharide chains. Evidence is reviewed to suggest that, in the wall of a living plant cell, Cu+ and H2O2 are formed by reactions involving ascorbate and its products, dehydroascorbate and oxalate. Systems may thus be in place to produce apoplastic .OH radicals in vivo. Although .OH radicals are often regarded as detrimental, they are so short-lived that they could act as site-specific oxidants targeted to play a useful role in loosening the cell wall, e.g. during cell expansion, fruit ripening and organ abscission.

摘要

一般认为植物细胞壁多糖在体内的断裂是由酶催化的。然而,在存在L-抗坏血酸的情况下,这些多糖在生理相关条件下会发生非酶促断裂。1 mM抗坏血酸对木葡聚糖的断裂作用在pH值为4.5时达到最佳,在延迟10 - 25分钟后达到最大断裂速率。过氧化氢酶可阻止这种断裂,而添加H2O2(0.1 - 10 mM)会增加断裂速率并缩短延迟时间。抗坏血酸在约5 microM以上可引起可检测到的木葡聚糖断裂。脱氢抗坏血酸的效果要差得多。添加Cu2+(>0.3 microM)也会增加抗坏血酸诱导的断裂速率;EDTA具有抑制作用。在不添加金属的情况下的断裂速率似乎归因于木葡聚糖中存在的痕量Cu(2.8 mg.kg-1)。抗坏血酸诱导的木葡聚糖断裂受到自由基清除剂的抑制;它们的有效性与其与羟基自由基(·OH)反应的速率常数成正比。有人提出抗坏血酸非酶促地将O2还原为H2O2,将Cu2+还原为Cu+,并且H2O2和Cu+反应形成·OH,从而导致多糖链的氧化断裂。有证据表明,在活植物细胞的细胞壁中,Cu+和H2O2是由涉及抗坏血酸及其产物脱氢抗坏血酸和草酸盐的反应形成的。因此,体内可能存在产生质外体·OH自由基的系统。尽管·OH自由基通常被认为是有害的,但它们寿命极短,因此可以作为位点特异性氧化剂,在例如细胞扩张、果实成熟和器官脱落过程中,在细胞壁松弛中发挥有益作用。

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