首页> 美国卫生研究院文献>other >Four tyrosine residues of the rice immune receptor XA21 are not required for interaction with the co-receptor OsSERK2 or resistance to Xanthomonas oryzae pv. oryzae
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Four tyrosine residues of the rice immune receptor XA21 are not required for interaction with the co-receptor OsSERK2 or resistance to Xanthomonas oryzae pv. oryzae

机译:水稻免疫受体XA21的四个酪氨酸残基与共受体OsSERK2相互作用或对米氏黄单胞菌(Xanthomonas oryzae pv)的抗性不需要。水稻

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摘要

Tyrosine phosphorylation has emerged as an important regulator of plasma membrane-localized immune receptors activity. Here, we investigate the role of tyrosine phosphorylation in the regulation of rice XANTHOMONAS RESISTANCE 21 (XA21)-mediated immunity. We demonstrate that the juxtamembrane and kinase domain of Escherichia coli–expressed XA21 (XA21JK) autophosphorylates on tyrosine residues. Directed mutagenesis of four out of the nine tyrosine residues in XA21JK reduced autophosphorylation. These sites include Tyr698 in the juxtamembrane domain, and Tyr786, Tyr907, and Tyr909 in the kinase domain. Rice plants expressing XA21-GFP fusion proteins or proteins with these tyrosine residues individually mutated to phenylalanine (XA21YF-GFP), which prevents phosphorylation at these sites, maintain resistance to Xanthomonas oryzae pv. oryzae. In contrast, plants expressing phosphomimetic XA21 variants with tyrosine mutated to aspartate (XA21YD-GFP) were susceptible. In vitro purified XA21JKY698F, XA21JKY907F, and XA21JKY909F variants are catalytically active, whereas activity was not detected in XA21JKY768F and the four XA21JKYD variants. We previously demonstrated that interaction of XA21 with the co-receptor OsSERK2 is critical for biological function. Four of the XA21JKYF variants maintain interaction with OsSERK2 as well as the XA21 binding (XB) proteins XB3 and XB15 in yeast, suggesting that these four tyrosine residues are not required for their interaction. Taken together, these results suggest that XA21 is capable of tyrosine autophosphorylation, but the identified tyrosine residues are not required for activation of XA21-mediated immunity or interaction with predicted XA21 signaling proteins.
机译:酪氨酸磷酸化已成为质膜定位免疫受体活性的重要调节剂。在这里,我们调查酪氨酸磷酸化在水稻黄单胞菌耐药性21(XA21)介导的免疫调节中的作用。我们证明大肠杆菌的近膜和激酶结构域在酪氨酸残基上表达了XA21(XA21JK)自磷酸化。 XA21JK的9个酪氨酸残基中有4个的定向诱变减少了自身磷酸化。这些位点包括近膜结构域中的Tyr 698 和Tyr 786 ,Tyr 907 和Tyr 909 激酶结构域。表达XA21-GFP融合蛋白或带有这些酪氨酸残基的蛋白分别突变为苯丙氨酸的水稻植株(XA21 YF -GFP)可防止这些位点的磷酸化,从而保持对米黄单胞菌的抗性。水稻相反,表达酪氨酸突变为天冬氨酸(XA21 YD -GFP)的拟磷酸化XA21变体的植物易感。体外纯化的XA21JK Y698F ,XA21JK Y907F 和XA21JK Y909F 变体具有催化活性,而在XA21JK Y768F < / sup>和四个XA21JK YD 变体。我们先前证明了XA21与共受体OsSERK2的相互作用对于生物学功能至关重要。 XA21JK YF 变体中的四个与酵母中的OsSERK2以及XA21结合(XB)蛋白XB3和XB15保持相互作用,这表明这四个酪氨酸残基不需要相互作用。综上所述,这些结果表明XA21能够进行酪氨酸自磷酸化,但是鉴定出的酪氨酸残基对于激活XA21介导的免疫或与预期的XA21信号蛋白相互作用不是必需的。

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