Abstract
Kinesin-like calmodulin-binding protein (KCBP) is a novel member of the kinesin superfamily that is involved in cell division and trichome morphogenesis. KCBP is unique among all known kinesins in having a myosin tail homology-4 region in the N-terminal tail and a calmodulin-binding region following the motor domain. Calcium, through calmodulin, has been shown to negatively regulate the interaction of KCBP with microtubules. Here we have used the yeast two-hybrid system to identify the proteins that interact with the tail region of KCBP. A protein kinase (KCBP-interacting protein kinase (KIPK)) was found to interact specifically with the tail region of KCBP. KIPK is related to a group of protein kinases specific to plants that has an additional sequence between subdomains VII and VIII of the conserved C-terminal catalytic domain and an extensive N-terminal region. The catalytic domain alone of KIPK interacted weakly with the N-terminal KCBP protein but strongly with full-length KCBP, whereas the noncatalytic region did not interact with either protein. The interaction of KCBP with KIPK was confirmed using coprecipitation assays. Using bacterially expressed full-length and truncated proteins, we have shown that the catalytic domain is capable of phosphorylating itself. The association of KIPK with KCBP suggests regulation of KCBP or KCBP-associated proteins by phosphorylation and/or that KCBP is involved in targeting KIPK to its proper cellular location.
Highlights
Kinesin and kinesin-like proteins (KLPs)1 are microtubulebased transport motor proteins that perform a variety of important cellular and developmental functions such as controlling steady-state structural organization of cytoplasm; moving and positioning of intracellular macromolecules and organelles; and driving cell movement, cell division, and flagellar movement [1,2,3]
Previous studies have shown that the C-terminal region of Kinesin-like calmodulin-binding protein (KCBP) interacts with microtubules, tubulin subunits, and calmodulin (22, 25, 28 –30, 47)
An A. thaliana cDNA library consisting of clones in probed with GAL4 AD monoclonal antibody (pACT) as fusions to the activation domain of Gal4 was screened using the aminoterminal domain of KCBP in pAS1CYH2 as a fusion to the DNA binding domain of Gal4
Summary
Sible for phosphorylation has not been established in all cases. Two kinases have been shown to phosphorylate specific KLPs. Using a PCR screen for kinesins in sea urchin, Rogers et al [31] isolated a kinesin (kinesin-C) with a calmodulin-binding domain It has sequence similarity in the motor and calmodulin-binding domains with KCBP, it does not contain the myosin tail homology-4 and talin-like regions present in the N-terminal portion of KCBP. Genetic studies have shown that SUZ2 may interact with ZWI (KCBP) and with FURCAI, a protein involved in trichome branching. These suppressor studies suggest that KCBP interacts with several other proteins in the cell [27, 40]. We have confirmed the interaction in vitro and have demonstrated autophosphorylation of KIPK
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