dissecting the sequential assembly and localization of intraflagellar transport particle complex b in chlamydomonas解剖intraflagellar运输粒子的顺序组装和定位复杂b在衣藻.pdfVIP
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dissecting the sequential assembly and localization of intraflagellar transport particle complex b in chlamydomonas解剖intraflagellar运输粒子的顺序组装和定位复杂b在衣藻
Dissecting the Sequential Assembly and Localization of
Intraflagellar Transport Particle Complex B in
Chlamydomonas
Elizabeth A. Richey, Hongmin Qin*
Department of Biology, Texas AM University, College Station, Texas, United States of America
Abstract
Intraflagellar transport (IFT), the key mechanism for ciliogenesis, involves large protein particles moving bi-directionally
along the entire ciliary length. IFT particles contain two large protein complexes, A and B, which are constructed with
proteins in a core and several peripheral proteins. Prior studies have shown that in Chlamydomonas reinhardtii, IFT46, IFT52,
and IFT88 directly interact with each other and are in a subcomplex of the IFT B core. However, ift46, bld1, and ift88 mutants
differ in phenotype as ift46 mutants are able to form short flagella, while the other two lack flagella completely. In this study,
we investigated the functional differences of these individual IFT proteins contributing to complex B assembly, stability, and
basal body localization. We found that complex B is completely disrupted in bld1 mutant, indicating an essential role of
IFT52 for complex B core assembly. Ift46 mutant cells are capable of assembling a relatively intact complex B, but such
complex is highly unstable and prone to degradation. In contrast, in ift88 mutant cells the complex B core still assembles
and remains stable, but the peripheral proteins no longer attach to the B core. Moreover, in ift88 mutant cells, while
complex A and the anterograde IFT motor FLA10 are localized normally to the transition fibers, complex B proteins instead
are accumulated at the proximal ends of the basal bodies. In addition, in bld2 mutant, the IFT complex B proteins still
localize to the proximal ends of defective centrioles which completely lack transition
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