Abstract
We have shown previously that only the long myosin light chain kinase (MLCK), which is the predominant MLCK isoform expressed in nonmuscle cells, localizes to the cleavage furrow. To further examine the in vivo localization of the long MLCK in HeLa cells and the mechanisms responsible for kinase targeting during the cell cycle, we examined the distribution of the endogenous kinase and constructed green fluorescent protein (GFP) fusions of long HeLa MLCK truncations. A GFP fusion containing the N-terminal IgG domain and the five DXR motifs localized to stress fibers during interphase and the cleavage furrow during mitosis. Although individual fusions of the five DXRs and IgG domain both independently localized to stress fibers, only the five DXRs demonstrated a cortical localization in mitotic cells. Thus, robust targeting of the long MLCK to the cleavage furrow required the five DXRs and additional sequences from the IgG domain. Expression of the IgG domain alone or with five DXRs increased the number of multinucleate cells tenfold, whereas expression of the five DXRs or GFP had no effect. Furthermore, expression of the IgG domain alone or with five DXRs disrupted normal spindle morphology during mitosis. Extended astral microtubules and increased bundling of kinetochore microtubules, and spindle pole fragmentation were detected in mitotic cells. These microtubule defects were associated with abnormalities in metaphase chromosome alignment and a subsequent metaphase arrest caused by activation of the spindle assembly checkpoint at the kinetochores of mono-oriented chromosomes. Together, these results suggest that MLCK has an unexpected regulatory function during mitosis.
Highlights
Biochemical studies have shown that phosphorylation on Ser19 of the regulatory light chain (RLC) of myosin-II takes place late in mitosis (Satterwhite et al, 1992; Yamakita et al, 1994), and studies using a myosin-II biosensor that monitors Ser-19 phosphorylation (DeBiasio et al, 1996) and Ser-19 phosphoepitope antibodies (Matsumura et al, 1998) confirmed these early observations
To examine further the mechanisms responsible for kinase targeting during the cell cycle, we evaluated the distribution of the endogenous kinase and constructed green fluorescent protein (GFP) fusions of HeLa long Myosin light chain kinase (MLCK) truncations
Distribution of the endogenous HeLa long MLCK To examine the distribution of the endogenous long MLCK, we fixed and stained untransfected HeLa cells with antibodies against the IgG domain of the HeLa long MLCK
Summary
Biochemical studies have shown that phosphorylation on Ser of the regulatory light chain (RLC) of myosin-II takes place late in mitosis (Satterwhite et al, 1992; Yamakita et al, 1994), and studies using a myosin-II biosensor that monitors Ser-19 phosphorylation (DeBiasio et al, 1996) and Ser-19 phosphoepitope antibodies (Matsumura et al, 1998) confirmed these early observations. Expression of an RLC with alanine substitutions at Ser-19 and Thr-18 induces multiple defects during mitosis (Komatsu et al, 2000). These in vivo studies emphasize the importance of Ser-19 phosphorylation during mitosis and indicate that activation of the myosin-II motor is an important regulatory step in cell division. Myosin light chain kinase (MLCK) is a leading candidate for mediating myosin-II phosphorylation during mitosis because it is a dedicated, Ca2+/calmodulin-regulated kinase that exclusively phosphorylates Thr-18 and Ser-19 on the regulatory light chain of myosin-II. MLCK-mediated phosphorylation of Ser-19 has been implicated in regulating a wide array of cellular functions (Kamm and Stull, 2001)
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