Buetow Lori, Tria Giancarlo, Ahmed Syed Feroj, Hock Andreas, Dou Hao, Sibbet Gary J, Svergun Dmitri I, Huang Danny T
Cancer Research UK Beatson Institute, Garscube Estate, Switchback Road, Glasgow, G61 1BD, UK.
EMBL c/o DESY, Notkestrasse 85, Geb, 25a, 22603, Hamburg, Germany.
BMC Biol. 2016 Sep 8;14(1):76. doi: 10.1186/s12915-016-0298-6.
Casitas B-lineage lymphoma (Cbl or c-Cbl) is a RING ubiquitin ligase that negatively regulates protein tyrosine kinase (PTK) signalling. Phosphorylation of a conserved residue (Tyr371) on the linker helix region (LHR) between the substrate-binding and RING domains is required to ubiquitinate PTKs, thereby flagging them for degradation. This conserved Tyr is a mutational hotspot in myeloproliferative neoplasms. Previous studies have revealed that select point mutations in Tyr371 can potentiate transformation in cells and mice but not all possible mutations do so. To trigger oncogenic potential, Cbl Tyr371 mutants must perturb the LHR-substrate-binding domain interaction and eliminate PTK ubiquitination. Although structures of native and pTyr371-Cbl are available, they do not reveal how Tyr371 mutations affect Cbl's conformation. Here, we investigate how Tyr371 mutations affect Cbl's conformation in solution and how this relates to Cbl's ability to potentiate transformation in cells.
To explore how Tyr371 mutations affect Cbl's properties, we used surface plasmon resonance to measure Cbl mutant binding affinities for E2 conjugated with ubiquitin (E2-Ub), small angle X-ray scattering studies to investigate Cbl mutant conformation in solution and focus formation assays to assay Cbl mutant transformation potential in cells. Cbl Tyr371 mutants enhance E2-Ub binding and cause Cbl to adopt extended conformations in solution. LHR flexibility, RING domain accessibility and transformation potential are associated with the extent of LHR-substrate-binding domain perturbation affected by the chemical nature of the mutation. More disruptive mutants like Cbl Y371D or Y371S are more extended and the RING domain is more accessible, whereas Cbl Y371F mimics native Cbl in solution. Correspondingly, the only Tyr371 mutants that potentiate transformation in cells are those that perturb the LHR-substrate-binding domain interaction.
c-Cbl's LHR mutations are only oncogenic when they disrupt the native state and fail to ubiquitinate PTKs. These findings provide new insights into how LHR mutations deregulate c-Cbl.
Casitas B 系淋巴瘤(Cbl 或 c-Cbl)是一种 RING 泛素连接酶,对蛋白酪氨酸激酶(PTK)信号传导起负调控作用。在底物结合域和 RING 域之间的连接螺旋区域(LHR)上,一个保守残基(Tyr371)的磷酸化是 PTK 泛素化所必需的,从而标记它们以供降解。这个保守的 Tyr 是骨髓增殖性肿瘤中的一个突变热点。先前的研究表明,Tyr371 中的某些点突变可增强细胞和小鼠中的转化能力,但并非所有可能的突变都如此。为了触发致癌潜能,Cbl Tyr371 突变体必须扰乱 LHR 与底物结合域的相互作用并消除 PTK 泛素化。尽管天然和 pTyr371-Cbl 的结构是已知的,但它们并未揭示 Tyr371 突变如何影响 Cbl 的构象。在此,我们研究 Tyr371 突变如何影响溶液中 Cbl 的构象,以及这与 Cbl 在细胞中增强转化的能力有何关系。
为了探究 Tyr371 突变如何影响 Cbl 的特性,我们使用表面等离子体共振来测量 Cbl 突变体与泛素偶联的 E2(E2-Ub)的结合亲和力,利用小角 X 射线散射研究来研究溶液中 Cbl 突变体构象,并通过集落形成试验来检测 Cbl 突变体在细胞中的转化潜能。Cbl Tyr371 突变体增强了 E2-Ub 结合,并使 Cbl 在溶液中呈现伸展构象。LHR 的灵活性、RING 域的可及性和转化潜能与受突变化学性质影响的 LHR-底物结合域扰动程度相关。像 Cbl Y371D 或 Y371S 这样更具破坏性的突变体更伸展,RING 域更易接近,而 Cbl Y371F 在溶液中模拟天然 Cbl。相应地,在细胞中增强转化的唯一 Tyr371 突变体是那些扰乱 LHR-底物结合域相互作用的突变体。
c-Cbl 的 LHR 突变只有在破坏天然状态且无法使 PTK 泛素化时才具有致癌性。这些发现为 LHR 突变如何使 c-Cbl 失调提供了新的见解。
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