Nicholas Matthew P, Berger Florian, Rao Lu, Brenner Sibylle, Cho Carol, Gennerich Arne
Department of Anatomy and Structural Biology, Gruss Lipper Biophotonics Center, and Medical Scientist Training Program, Albert Einstein College of Medicine, Bronx, NY 10461;
Theory and Bio-Systems, Max Planck Institute of Colloids and Interfaces, 14424 Potsdam, Germany; Laboratory of Sensory Neuroscience, and Howard Hughes Medical Institute, Rockefeller University, New York, NY 10065; and.
Proc Natl Acad Sci U S A. 2015 May 19;112(20):6371-6. doi: 10.1073/pnas.1417422112. Epub 2015 May 4.
Cytoplasmic dynein is a homodimeric microtubule (MT) motor protein responsible for most MT minus-end-directed motility. Dynein contains four AAA+ ATPases (AAA: ATPase associated with various cellular activities) per motor domain (AAA1-4). The main site of ATP hydrolysis, AAA1, is the only site considered by most dynein motility models. However, it remains unclear how ATPase activity and MT binding are coordinated within and between dynein's motor domains. Using optical tweezers, we characterize the MT-binding strength of recombinant dynein monomers as a function of mechanical tension and nucleotide state. Dynein responds anisotropically to tension, binding tighter to MTs when pulled toward the MT plus end. We provide evidence that this behavior results from an asymmetrical bond that acts as a slip bond under forward tension and a slip-ideal bond under backward tension. ATP weakens MT binding and reduces bond strength anisotropy, and unexpectedly, so does ADP. Using nucleotide binding and hydrolysis mutants, we show that, although ATP exerts its effects via binding AAA1, ADP effects are mediated by AAA3. Finally, we demonstrate "gating" of AAA1 function by AAA3. When tension is absent or applied via dynein's C terminus, ATP binding to AAA1 induces MT release only if AAA3 is in the posthydrolysis state. However, when tension is applied to the linker, ATP binding to AAA3 is sufficient to "open" the gate. These results elucidate the mechanisms of dynein-MT interactions, identify regulatory roles for AAA3, and help define the interplay between mechanical tension and nucleotide state in regulating dynein motility.
胞质动力蛋白是一种同型二聚体微管(MT)运动蛋白,负责大多数微管负端定向运动。动力蛋白每个运动结构域含有四个AAA+ATP酶(AAA:与各种细胞活动相关的ATP酶)(AAA1-4)。ATP水解的主要位点AAA1是大多数动力蛋白运动模型考虑的唯一位点。然而,动力蛋白运动结构域内部和之间的ATP酶活性与微管结合是如何协调的仍不清楚。我们使用光镊表征了重组动力蛋白单体的微管结合强度与机械张力和核苷酸状态的函数关系。动力蛋白对张力呈各向异性响应,当朝着微管正端拉动时与微管结合更紧密。我们提供的证据表明,这种行为源于一种不对称键,该键在向前张力下作为滑动键,在向后张力下作为滑动理想键。ATP会削弱微管结合并降低键强度各向异性,出乎意料的是,ADP也会如此。使用核苷酸结合和水解突变体,我们表明,尽管ATP通过结合AAA1发挥其作用,但ADP的作用是由AAA3介导的。最后,我们证明了AAA3对AAA1功能的“门控”作用。当不存在张力或通过动力蛋白的C末端施加张力时,只有当AAA3处于水解后状态时,ATP与AAA1的结合才会诱导微管释放。然而,当对连接体施加张力时,ATP与AAA3的结合足以“打开”门。这些结果阐明了动力蛋白与微管相互作用的机制,确定了AAA3的调节作用,并有助于定义机械张力和核苷酸状态在调节动力蛋白运动中的相互作用。