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两种不同形式的M位点蛋白激酶定位于质膜,并直接与S位点受体激酶相互作用,以转导白菜中的自交不亲和信号。

Two distinct forms of M-locus protein kinase localize to the plasma membrane and interact directly with S-locus receptor kinase to transduce self-incompatibility signaling in Brassica rapa.

作者信息

Kakita Mitsuru, Murase Kohji, Iwano Megumi, Matsumoto Tomohito, Watanabe Masao, Shiba Hiroshi, Isogai Akira, Takayama Seiji

机构信息

Graduate School of Biological Sciences, Nara Institute of Science and Technology, 8916-5 Takayama, Ikoma 630-0192, Japan.

出版信息

Plant Cell. 2007 Dec;19(12):3961-73. doi: 10.1105/tpc.106.049999. Epub 2007 Dec 7.

Abstract

Many flowering plants possess systems of self-incompatibility (SI) to prevent inbreeding. In Brassica, SI recognition is controlled by the multiallelic gene complex (S-haplotypes) at the S-locus, which encodes both the male determinant S-locus protein 11 (SP11/SCR) and the female determinant S-receptor kinase (SRK). Upon self-pollination, the S-haplotype-specific interaction between the pollen-borne SP11 and the cognate stigmatic SRK receptor induces SI signaling in the stigmatic papilla cell and results in rejection of the self-pollen. Our genetic analysis of a self-compatible mutant revealed the involvement of a cytoplasmic protein kinase, M-locus protein kinase (MLPK), in the SI signaling, but its exact physiological function remains unknown. In this study, we identified two different MLPK transcripts, MLPKf1 and MLPKf2, which are produced using alternative transcriptional initiation sites and encode two isoforms that differ only at the N termini. While MLPKf1 and MLPKf2 exhibited distinct expression profiles, both were expressed in papilla cells. MLPKf1 localizes to the plasma membrane through its N-terminal myristoylation motif, while MLPKf2 localizes to the plasma membrane through its N-terminal hydrophobic region. Although both MLPKf1 and MLPKf2 could independently complement the mlpk/mlpk mutation, their mutant forms that lack the plasma membrane localization motifs failed to complement the mutation. Furthermore, a bimolecular fluorescence complementation assay revealed direct interactions between SRK and the MLPK isoforms in planta. These results suggest that MLPK isoforms localize to the papilla cell membrane and interact directly with SRK to transduce SI signaling.

摘要

许多开花植物拥有防止近亲繁殖的自交不亲和(SI)系统。在芸苔属植物中,SI识别由位于S位点的多等位基因复合体(S单倍型)控制,该复合体编码雄性决定因子S位点蛋白11(SP11/SCR)和雌性决定因子S受体激酶(SRK)。自花授粉时,花粉携带的SP11与同源柱头SRK受体之间的S单倍型特异性相互作用在柱头乳头细胞中诱导SI信号传导,导致自花花粉被排斥。我们对一个自交亲和突变体的遗传分析揭示了一种细胞质蛋白激酶,即M位点蛋白激酶(MLPK)参与了SI信号传导,但其确切的生理功能仍然未知。在本研究中,我们鉴定出两种不同的MLPK转录本,MLPKf1和MLPKf2,它们通过不同的转录起始位点产生,编码仅在N末端不同的两种同工型。虽然MLPKf1和MLPKf2表现出不同的表达谱,但两者都在乳头细胞中表达。MLPKf1通过其N末端肉豆蔻酰化基序定位于质膜,而MLPKf2通过其N末端疏水区域定位于质膜。尽管MLPKf1和MLPKf2都能独立地互补mlpk/mlpk突变,但缺乏质膜定位基序的它们的突变形式无法互补该突变。此外,双分子荧光互补分析揭示了SRK与植物中MLPK同工型之间的直接相互作用。这些结果表明,MLPK同工型定位于乳头细胞膜并与SRK直接相互作用以转导SI信号。

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