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Instytut Biologii Doświadczalnej im. Marcelego Nenckiego PAN.
Contributor:Kasprzak, Andrzej : Supervisor
Publisher:Instytut Biologii Doświadczalnej im. M. Nenckiego PAN
Place of publishing: Date issued/created: Description:205 pages : illustrations ; 30 cm + 1 CD ; Bibliography ; Summary in English
Degree grantor:Instytut Biologii Doświadczalnej im. Marcelego Nenckiego PAN
Type of object: Subject and Keywords:Kinesin-1 ; Microtubule ; Microtubule-microtubule sliding
Abstract:Kinesin-1 is a motor protein that converts energy from ATP hydrolysis into mechanical movement. This motor protein "walks" on the microtubule (MT) towards its plus end. Kinesin-1 is a heterotetramer composed of two heavy chains and two light chains. The heavy chain consists of a motor domain (amino terminus) containing a catalytic center, a neck linker, a coiled-coil domain and, at the carboxy terminus, a tail which is responsible for cargo binding. The main role of kinesin-1 in cells is to transport various cargoes from the cell body to its distal parts and to reorganize the microtubular cytoskeleton.The two kinesin-1 heavy chains contain two MT binding sites - one in the motor domain, and the other in the tail. As a result, kinesin-1 can simultaneously interact with two MTs, and cross-link them or move them against each other. In the neuron, this process is necessary during axon formation - mechanical pressure on the cell membrane initiates and directs the formation of a neurite. However, still little is known about the mechanism of MT sliding by kinesin-1, the mutual orientation of the MTs during movement, the way kinesin molecules bind between the MTs, and the regulation of these processes.In order to investigate the mechanism of MT-pair sliding driven by kinesin-1, a new in vitro motility assay was developed. Full length recombinant dimeric kinesin-1 without light chains was tested. Both kinesin-1 and MTs were marked with fluorescent dyes which enabled their individual observation and visualization using a total internal reflection microscopy (TIRFM). This technique allowed the simultaneous observation of the kinesin-1 as well as the cargo MT and stationary MT, which contained different proportions of the fluorescent dye in order to distinguish them from each other.Analysis of the movies obtained from TIRFM showed that the average velocity of MT-MT sliding by kinesin-1 (120 nm/s) is much lower than for kinesin-1 single molecules (600 nm/s) or in gliding assay (1200 nm/s). Contrary to the other two analyzes, MT-MT sliding was not smooth, there were visible breaks in movement, and there were often significant interruptions during MT transport. Experiments with polarity marked MTs showed that there were 3 ways of MT-MT sliding and stationary MT orientation: sliding of the anti-parallel MTs to the plus end, parallel MT sliding towards the minus end, and parallel sliding to the plus end of the stationary MT. Unexpectedly, it turned out that not only anti-parallel MTs are transported, as observed for other motor proteins, but also parallel MTs, which, according to the mechanism suggested in this thesis, is the result of the processive generation of movement by kinesin-1.Kinesin-1 can undergo autoinhibition – a change in conformation that prevents movement, which could make it difficult to repeatedly observe the process of MT sliding. To eliminate the flexible kinesin fragment necessary for autoinhibition (molecular hinge- 2, Δ505-610), a construct lacking hinge-2 was created using molecular biology tools. It turned out that hingeless kinesin-1 performed MT-pair sliding 6 times less frequently, with run length 5 times lower comparing to wild-type kinesin-1. Thus, the presence of an elastic fragment is necessary to compensate the lack of synchronization among the kinesin-1 molecules transporting the same MT.The effect of post-translational modifications of tubulin on MT-MT sliding by kinesin-1 was also investigated. It has been shown that for detyrosinated microtubules, the duration of the movement is longer than for the tyrosinated ones. Concerning glutamylation of microtubules, a lower percentage of movement interruptions was observed as compared to the control. On the other hand, the analysis of the velocity and run length of transport showed no significant effects of the post-translational modifications of tubulin investigated here
Resource type: Detailed Resource Type: Source: Language: Language of abstract: Digitizing institution:Nencki Institute of Experimental Biology of the Polish Academy of Sciences
Original in:Library of the Nencki Institute of Experimental Biology PAS
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