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BDP-30是一种来自白花丹的系统抗性诱导剂,可抑制烟草花叶病毒感染,并与核糖体失活蛋白具有同源性。

BDP-30, a systemic resistance inducer from Boerhaavia diffusa L., suppresses TMV infection, and displays homology with ribosome-inactivating proteins.

作者信息

Srivastava Shalini, Verma H N, Srivastava Aparana, Prasad Vivek

机构信息

Molecular Plant Virology Lab, Department of Botany, Lucknow University, Lucknow 226 007, India.

出版信息

J Biosci. 2015 Mar;40(1):125-35. doi: 10.1007/s12038-014-9494-0.

Abstract

Root extract of Boerhaavia diffusa L. induced systemic resistance in tobacco against Tobacco mosaic virus. A 30 kDa protein was isolated as the active component, called BDP-30 on the basis of the molecular weight and source plant. BDP-30, a glycoprotein, was found to be temperature and protease resistant. It was basic, possessing a pI greater than 9.0. In-gel proteolytic digestion of BDP-30 generated two peptides that possessed the amino acid sequence KLYDIPPLR and KVTLPYSGNYER by LC/MS/MS. Both peptides shared absolute sequence identity with trichosanthin, a ribosome-inactivating protein from Trichosanthes kirilowii, and a 78 percent and 100 percent homology respectively with an RIP from Bryonia dioica, bryodin. Further, effort was made to look at the fate of TMV in induced resistant Nicotiana tabacum cv. Xanthi, a systemic host of the virus, at specified days after inoculation in control and treated plants. TMV coat protein (CP) was detected by immunoblot 7 days post inoculation up to 21 days in the control set, but not in treated resistant plants. TMV RNA was detected by RT-PCR using TMV-CP specific primers. Resistant tobacco did not show presence of TMV RNA up to 21 days of inoculation. This suggests that BDP-30 may be suppressing TMV replication.

摘要

白花蛇舌草根提取物诱导烟草对烟草花叶病毒产生系统抗性。分离出一种30 kDa的蛋白质作为活性成分,根据分子量和来源植物将其命名为BDP - 30。BDP - 30是一种糖蛋白,具有耐温度和蛋白酶的特性。它呈碱性,pI大于9.0。通过LC/MS/MS对BDP - 30进行凝胶内蛋白水解消化产生了两个肽段,其氨基酸序列分别为KLYDIPPLR和KVTLPYSGNYER。这两个肽段与天花粉蛋白(一种来自瓜蒌的核糖体失活蛋白)具有完全相同的序列,并且分别与来自白泻根的核糖体失活蛋白bryodin具有78%和100%的同源性。此外,还研究了烟草花叶病毒在诱导抗性的烟草品种Xanthi(该病毒的系统寄主)中的命运,在接种后的特定天数观察对照植株和处理植株的情况。接种后7天至21天,在对照植株中通过免疫印迹法检测到烟草花叶病毒外壳蛋白(CP),但在处理后的抗性植株中未检测到。使用烟草花叶病毒CP特异性引物通过RT - PCR检测烟草花叶病毒RNA。在接种后长达21天的抗性烟草中未检测到烟草花叶病毒RNA。这表明BDP - 30可能抑制了烟草花叶病毒的复制。

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