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Differential Elicitation of Two Processing Proteases Controls the Processing Pattern of the Trypsin Proteinase Inhibitor Precursor in Nicotiana attenuata1

机译:两种加工蛋白酶的差异性诱导控制了烟草中胰蛋白酶抑制因子前体的加工模式。

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Trypsin proteinase inhibitors (TPIs) of Nicotiana attenuata are major antiherbivore defenses that increase dramatically in leaves after attack or methyl jasmonate (MeJA) elicitation. To understand the elicitation process, we characterized the proteolytic fragmentation and release of TPIs from a multidomain precursor by proteases in MeJA-elicited and unelicited plants. A set of approximately 6-kD TPI peptides was purified from leaves, and their posttranslational modifications were characterized. In MeJA-elicited plants, the diversity of TPI structures was greater than the precursor gene predicted. This elicited structural heterogeneity resulted from differential fragmentation of the linker peptide (LP) that separates the seven-domain TPI functional domains. Using an in vitro fluorescence resonance energy transfer assay and synthetic substrates derived from the LP sequence, we characterized proteases involved in both the processing of the TPI precursor and its vacuolar targeting sequence. Although both a vacuolar processing enzyme and a subtilisin-like protease were found to participate in a two-step processing of LP, only the activity of the subtilisin-like protease was significantly increased by MeJA elicitation. We propose that MeJA elicitation increases TPI precursor production and saturates the proteolytic machinery, changing the processing pattern of TPIs. To test this hypothesis, we elicited a TPI-deficient N. attenuata genotype that had been transformed with a functional NaTPI gene under control of a constitutive promoter and characterized the resulting TPIs. We found no alterations in the processing pattern predicted from the sequence: a result consistent with the saturation hypothesis.
机译:弱烟烟草的胰蛋白酶蛋白酶抑制剂(TPIs)是主要的抗草食动物防御能力,在攻击或茉莉酸甲酯(MeJA)诱导后,叶片中的防御酶含量急剧增加。为了理解诱导过程,我们表征了蛋白酶在MeJA诱导和未诱导植物中通过多域前体产生的蛋白水解片段化和TPIs释放。从叶中纯化出一组大约6 kD TPI肽,并对其翻译后修饰进行了表征。在MeJA诱导的植物中,TPI结构的多样性大于预期的前体基因。这引起结构异质性是由于连接肽(LP)的差异性片段所致,该片段将七个结构域的TPI功能域分开。使用体外荧光共振能量转移测定法和源自LP序列的合成底物,我们表征了参与TPI前体及其液泡靶向序列加工的蛋白酶。尽管发现液泡加工酶和枯草杆菌蛋白酶样蛋白酶都参与了LP的两步加工,但是MeJA诱导仅使枯草杆菌蛋白酶样蛋白酶的活性显着增加。我们建议MeJA激发增加TPI前体的产量并饱和蛋白水解机制,从而改变TPI的加工方式。为了验证这一假设,我们引出了一个TPI缺陷型弱毒猪笼草基因型,该基因型已在功能性启动子的控制下被功能性NaTPI基因转化,并表征了产生的TPI。我们发现序列预测的处理模式没有变化:与饱和度假设一致的结果。

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