Schmidt Christian, Kim Dongkyoon, Ippolito Gregory C, Naqvi Hassan R, Probst Loren, Mathur Shawn, Rosas-Acosta German, Wilson Van G, Oldham Athenia L, Poenie Martin, Webb Carol F, Tucker Philip W
Institute for Cellular and Molecular Biology, The University of Texas at Austin, Austin, TX 78712, USA.
EMBO J. 2009 Mar 18;28(6):711-24. doi: 10.1038/emboj.2009.20. Epub 2009 Feb 12.
Regulation of BCR signalling strength is crucial for B-cell development and function. Bright is a B-cell-restricted factor that complexes with Bruton's tyrosine kinase (Btk) and its substrate, transcription initiation factor-I (TFII-I), to activate immunoglobulin heavy chain gene transcription in the nucleus. Here we show that a palmitoylated pool of Bright is diverted to lipid rafts of resting B cells where it associates with signalosome components. After BCR ligation, Bright transiently interacts with sumoylation enzymes, blocks calcium flux and phosphorylation of Btk and TFII-I and is then discharged from lipid rafts as a Sumo-I-modified form. The resulting lipid raft concentration of Bright contributes to the signalling threshold of B cells, as their sensitivity to BCR stimulation decreases as the levels of Bright increase. Bright regulates signalling independent of its role in IgH transcription, as shown by specific dominant-negative titration of rafts-specific forms. This study identifies a BCR tuning mechanism in lipid rafts that is regulated by differential post-translational modification of a transcription factor with implications for B-cell tolerance and autoimmunity.
BCR信号强度的调节对于B细胞的发育和功能至关重要。Bright是一种B细胞限制性因子,它与布鲁顿酪氨酸激酶(Btk)及其底物转录起始因子-I(TFII-I)形成复合物,以激活细胞核中的免疫球蛋白重链基因转录。我们在此表明,棕榈酰化的Bright池被转移至静息B细胞的脂筏中,在那里它与信号小体成分相关联。BCR连接后,Bright与类泛素化酶短暂相互作用,阻断钙通量以及Btk和TFII-I的磷酸化,然后以类泛素化修饰的形式从脂筏中排出。由此产生的Bright在脂筏中的浓度有助于B细胞的信号阈值,因为随着Bright水平的增加,它们对BCR刺激的敏感性降低。如通过对脂筏特异性形式进行特异性显性负向滴定所示,Bright独立于其在IgH转录中的作用来调节信号传导。这项研究确定了脂筏中的一种BCR调节机制,该机制由转录因子的差异翻译后修饰所调控,这对B细胞耐受性和自身免疫具有重要意义。
