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    Date Issued2009 (3)AuthorIkebe, Mitsuo (3)
    Sakai, Tsuyoshi (3)
    Lechtreck, Karl-Ferdinand (2)Witman, George B. (2)Ballif, Bryan A. (1)View MoreUMass Chan AffiliationDepartment of Cell Biology (3)Department of Physiology (3)Program in Molecular Medicine (2)Document TypeJournal Article (3)KeywordAnimals (2)Axoneme (2)Cell Biology (2)Chlamydomonas reinhardtii (2)Flagella (2)View MoreJournalMethods in cell biology (1)Proceedings of the National Academy of Sciences of the United States of America (1)The Journal of cell biology (1)

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    The Chlamydomonas reinhardtii BBSome is an IFT cargo required for export of specific signaling proteins from flagella

    Lechtreck, Karl-Ferdinand; Johnson, Eric C.; Sakai, Tsuyoshi; Cochran, Deborah A.; Ballif, Bryan A.; Rush, John; Pazour, Gregory J.; Ikebe, Mitsuo; Witman, George B. (2009-12-30)
    In humans, seven evolutionarily conserved genes that cause the cilia-related disorder Bardet-Biedl syndrome (BBS) encode proteins that form a complex termed the BBSome. The function of the BBSome in the cilium is not well understood. We purified a BBSome-like complex from Chlamydomonas reinhardtii flagella and found that it contains at least BBS1, -4, -5, -7, and -8 and undergoes intraflagellar transport (IFT) in association with a subset of IFT particles. C. reinhardtii insertional mutants defective in BBS1, -4, and -7 assemble motile, full-length flagella but lack the ability to phototax. In the bbs4 mutant, the assembly and transport of IFT particles are unaffected, but the flagella abnormally accumulate several signaling proteins that may disrupt phototaxis. We conclude that the BBSome is carried by IFT but is an adapter rather than an integral component of the IFT machinery. C. reinhardtii BBS4 may be required for the export of signaling proteins from the flagellum via IFT.
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    The tail binds to the head-neck domain, inhibiting ATPase activity of myosin VIIA

    Umeki, Nobuhisa; Jung, HyunSuk; Watanabe, Shinya; Sakai, Tsuyoshi; Li, Xiang-Dong; Ikebe, Reiko; Craig, Roger W.; Ikebe, Mitsuo (2009-05-09)
    Myosin VIIA is an unconventional myosin, responsible for human Usher syndrome type 1B, which causes hearing and visual loss. Here, we studied the molecular mechanism of regulation of myosin VIIA, which is currently unknown. Although it was originally thought that myosin VIIA is a dimeric myosin, our electron microscopic (EM) observations revealed that full-length Drosophila myosin VIIA (DM7A) is a monomer. Interestingly, the tail domain markedly inhibits the actin-activated ATPase activity of tailless DM7A at low Ca(2+) but not high Ca(2+). By examining various deletion constructs, we found that deletion of the distal IQ domain, the C-terminal region of the tail, and the N-terminal region of the tail abolishes the tail-induced inhibition of ATPase activity. Single-particle EM analysis of full-length DM7A at low Ca(2+) suggests that the tail folds back on to the head, where it contacts both the motor core domain and the neck domain, forming an inhibited conformation. We concluded that unconventional myosin that may be present a monomer in the cell can be regulated by intramolecular interaction of the tail with the head.
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    Total internal reflection fluorescence (TIRF) microscopy of Chlamydomonas flagella

    Engel, Benjamin D.; Lechtreck, Karl-Ferdinand; Sakai, Tsuyoshi; Ikebe, Mitsuo; Witman, George B.; Marshall, Wallace F. (2009-01-01)
    The eukaryotic flagellum is host to a variety of dynamic behaviors, including flagellar beating, the motility of glycoproteins in the flagellar membrane, and intraflagellar transport (IFT), the bidirectional traffic of protein particles between the flagellar base and tip. IFT is of particular interest, as it plays integral roles in flagellar length control, cell signaling, development, and human disease. However, our ability to understand dynamic flagellar processes such as IFT is limited in large part by the fidelity with which we can image these behaviors in living cells. This chapter introduces the application of total internal reflection fluorescence (TIRF) microscopy to visualize the flagella of Chlamydomonas reinhardtii. The advantages and challenges of TIRF are discussed in comparison to confocal and differential interference contrast techniques. This chapter also reviews current IFT insights gleaned from TIRF microscopy of Chlamydomonas and provides an outlook on the future of the technique, with particular emphasis on combining TIRF with other emerging imaging technologies.
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