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真菌β-葡聚糖片段与大豆(Glycine max L.)微粒体组分和原生质体的高亲和力结合。

High-affinity binding of fungal beta-glucan fragments to soybean (Glycine max L.) microsomal fractions and protoplasts.

作者信息

Cosio E G, Pöpperl H, Schmidt W E, Ebel J

机构信息

Institut für Biologie II der Universität, Lehrstuhl für Biochemie der Pflanzen, Freiburg, Federal Republic of Germany.

出版信息

Eur J Biochem. 1988 Aug 1;175(2):309-15. doi: 10.1111/j.1432-1033.1988.tb14198.x.

Abstract

We have recently reported the existence of binding sites in soybean membranes for a beta-glucan fraction derived from the fungal pathogen Phytophthora megasperma f. sp. glycinea, which may play a role in the elicitor-mediated phytoalexin response of this plant [Schmidt, W. E. & Ebel, J. (1987) Proc. Natl Acad. Sci. USA 84, 4117-4121]. The specificity of beta-glucan binding to soybean membranes has now been investigated using a variety of competing polyglucans and oligoglucans of fungal origin. P. megasperma beta-glucan binding showed high apparent affinity for branched glucans with degrees of polymerization greater than 12. Binding affinity showed good correlation with elicitor activity as measured in a soybean cotyledon bioassay. Modification of the glucans at the reducing end with phenylalkylamine reagents had no effect on binding affinity. This characteristic was used to synthesize an oligoglucosyl tyramine derivative suitable for radioiodination. The 125I-glucan (15-30 Ci/mmol) provided higher sensitivity and lower detection limits for the binding assays while behaving in a manner identical to the [3H]glucan used previously. More accurate determinations of the Kd value for glucan binding indicated a higher affinity than previously shown (37 nM versus 200 nM). The 125I-glucan was used to provide the first reported evidence of specific binding of a fungal beta-glucan fraction in vivo to soybean protoplasts. The binding affinity to protoplasts proved identical to that found in microsomal fractions.

摘要

我们最近报道了大豆膜中存在来自真菌病原体大豆疫霉f. sp. glycinea的β-葡聚糖组分的结合位点,其可能在该植物的激发子介导的植保素反应中发挥作用[施密特,W. E. & 埃贝尔,J. (1987年) 《美国国家科学院院刊》84, 4117 - 4121]。现在已使用多种源自真菌的竞争性多聚糖和低聚糖研究了β-葡聚糖与大豆膜结合的特异性。大豆疫霉β-葡聚糖结合对聚合度大于12的分支葡聚糖表现出高表观亲和力。结合亲和力与在大豆子叶生物测定中测得的激发子活性具有良好的相关性。用苯烷基胺试剂在还原端修饰葡聚糖对结合亲和力没有影响。利用这一特性合成了一种适用于放射性碘化的低聚葡萄糖基酪胺衍生物。125I-葡聚糖(15 - 30 Ci/mmol)为结合测定提供了更高的灵敏度和更低的检测限,同时其行为方式与先前使用的[3H]葡聚糖相同。对葡聚糖结合的Kd值进行更准确的测定表明其亲和力比先前显示的更高(37 nM对200 nM)。125I-葡聚糖被用于提供首个关于真菌β-葡聚糖组分在体内与大豆原生质体特异性结合的报道证据。对原生质体的结合亲和力被证明与在微粒体组分中发现的相同。

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