Chang W P, Ye Y, Clevenger C V
Department of Pathology and Laboratory Medicine, University of Pennsylvania Medical Center, Philadelphia 19104, USA.
Mol Cell Biol. 1998 Feb;18(2):896-905. doi: 10.1128/MCB.18.2.896.
The intracellular domain of the prolactin (PRL) receptor (PRLr) is required for PRL-induced signaling and proliferation. To identify and test the functional stoichiometry of those PRLr motifs required for transduction and growth, chimeras consisting of the extracellular domain of either the alpha or beta subunit of human granulocyte-macrophage colony-stimulating factor (GM-CSF) receptor (GM-CSFr) and the intracellular domain of the rat PRLr were synthesized. Because the high-affinity binding of GM-CSF results from the specific pairing of one alpha- and one beta-GM-CSFr, use of GM-CSFr/PRLr chimera enabled targeted dimerization of the PRLr intracellular domain. To that end, the extracellular domains of the alpha- and beta-GM-CSFr were conjugated to one of the following mutations: (i) PRLr C-terminal truncations, termed alpha278, alpha294, alpha300, alpha322, or beta322; (ii) PRLr tyrosine replacements, termed Y309F, Y382F, or Y309+382F; or, (iii) PRLr wild-type short, intermediate, or long isoforms. These chimeras were cotransfected into the cytokine-responsive Ba/F3 line, and their expression was confirmed by ligand binding and Northern and Western blot analyses. Data from these studies revealed that heterodimeric complexes of the wild type with C-terminal truncation mutants of the PRLr intracellular domain were incapable of ligand-induced signaling or proliferation. Replacement of any single tyrosine residue (Y309F or Y382F) in the dimerized PRLr complex resulted in a moderate reduction of receptor-associated Jak2 activation and proliferation. In contrast, trans replacement of these residues (i.e., alphaY309F and betaY382F) markedly reduced ligand-driven Jak2 activation and proliferation, while cis replacement of both tyrosine residues in a single intracellular domain (i.e., alphaY309+382F) produced an inactive signaling complex. Analysis of these GM-CSFr-PRLr complexes revealed equivalent levels of Jak2 in association with the mutant receptor chains, suggesting that the tyrosine residues at 309 and 382 do not contribute to Jak association, but instead to its activation. Heterodimeric pairings of the intracellular domains from the known PRLr receptor isoforms (short-intermediate, short-long, and intermediate-long) also yielded inactive receptor complexes. These data demonstrate that the tyrosine residues at 309 and 382, as well as additional residues within the C terminus of the dimerized PRLr complex, contribute to PRL-driven signaling and proliferation. Furthermore, these findings indicate a functional requirement for the pairing of Y309 and Y382 in trans within the dimerized receptor complex.
催乳素(PRL)受体(PRLr)的细胞内结构域是PRL诱导信号传导和细胞增殖所必需的。为了鉴定和测试转导及生长所需的那些PRLr基序的功能化学计量,合成了由人粒细胞 - 巨噬细胞集落刺激因子(GM - CSF)受体(GM - CSFr)的α或β亚基的细胞外结构域与大鼠PRLr的细胞内结构域组成的嵌合体。由于GM - CSF的高亲和力结合是由一个α - 和一个β - GM - CSFr的特异性配对产生的,使用GM - CSFr / PRLr嵌合体能够使PRLr细胞内结构域靶向二聚化。为此,将α - 和β - GM - CSFr的细胞外结构域与以下突变之一缀合:(i)PRLr C末端截短,称为α278、α294、α300、α322或β322;(ii)PRLr酪氨酸替代,称为Y309F、Y382F或Y309 + 382F;或(iii)PRLr野生型短、中或长亚型。将这些嵌合体共转染到细胞因子反应性Ba / F3细胞系中,并通过配体结合以及Northern和Western印迹分析确认它们的表达。这些研究的数据表明,野生型与PRLr细胞内结构域的C末端截短突变体的异二聚体复合物不能进行配体诱导的信号传导或细胞增殖。在二聚化的PRLr复合物中替换任何单个酪氨酸残基(Y309F或Y382F)会导致受体相关的Jak2激活和细胞增殖适度降低。相反,这些残基的反式替换(即αY309F和βY382F)显著降低配体驱动的Jak2激活和细胞增殖,而在单个细胞内结构域中顺式替换两个酪氨酸残基(即αY309 + 382F)产生无活性的信号复合物。对这些GM - CSFr - PRLr复合物的分析显示与突变受体链相关的Jak2水平相当,表明309和382位的酪氨酸残基对Jak结合没有贡献,而是对其激活有贡献。已知PRLr受体亚型(短 - 中、短 - 长和中 - 长)的细胞内结构域的异二聚体配对也产生无活性的受体复合物。这些数据表明,309和382位的酪氨酸残基以及二聚化的PRLr复合物C末端内的其他残基对PRL驱动的信号传导和细胞增殖有贡献。此外,这些发现表明在二聚化受体复合物中Y309和Y382反式配对的功能要求。
