A calmodulin-related light chain from fission yeast that functions with myosin-I and PI 4-kinase

Sammons, Matthew R.; James, Michael L.; Clayton, Joseph E.; Sladewski, Thomas E.; Sirotkin, Vladimir; Lord, Matthew

doi:10.1242/jcs.067850

Cited by 18 publications

(30 citation statements)

References 93 publications

Supporting

Mentioning

Contrasting

Unclassified

Order By: Relevance

“…This is a unifying hypothesis, given the well-established role of F-BAR proteins such as Cdc15p in clathrin-mediated endocytosis (Arasada and Pollard, 2011; Berro et al, 2010; Qualmann and Kelly, 2000; Tsujita et al, 2006). This hypothesis is consistent with previous evidence that Bgs1p is transported through the secretory pathway, such as Brefeldin A inhibiting the concentration of GFP-Bgs1p in the cleavage furrow (Liu et al, 2002) and genetic interactions between mutations in cytokinesis genes and genes required for membrane traffic through the Golgi apparatus (Park et al, 2009; Sammons et al, 2011; Walch-Solimena and Novick, 1999). Similarly, mutations in conserved genes required for vesicular transport in the Golgi apparatus (De Matteis and Luini, 2008; Jaulin et al, 2007; Valente et al, 2012) cause septation defects in fission yeast (Brazer et al, 2000; Mishra et al, 2005).…”

Section: Discussionsupporting

confidence: 92%

Contractile Ring Stability in S. pombe Depends on F-BAR Protein Cdc15p and Bgs1p Transport from the Golgi Complex

2014

View full text Add to dashboard Cite

Summary Cdc15p is known to contribute to cytokinesis in fission yeast; however, the protein is not required to assemble the contractile ring of actin and myosin, but helps to anchor the ring to the plasma membrane. Cdc15p has a lipid binding F-BAR domain, suggesting that it provides a physical link between the plasma membrane and contractile ring proteins. However, we find that a more important function of Cdc15p during cytokinesis is to help deliver a transmembrane enzyme, Bgs1p (also called Cps1p), from the Golgi apparatus to the plasma membrane, where it appears to anchor the contractile ring. Bgs1p synthesizes the cell wall in the cleavage furrow, but its enzyme activity is not required to anchor the contractile ring. We estimate that ~2000 Bgs1p molecules are required to anchor the ring. Without Bgs1p anchors, contractile rings slide along the plasma membrane, a phenomenon that depends on an unconventional type II myosin called Myp2p.

show abstract

Section: Discussionsupporting

confidence: 92%

Contractile Ring Stability in S. pombe Depends on F-BAR Protein Cdc15p and Bgs1p Transport from the Golgi Complex

2014

View full text Add to dashboard Cite

show abstract

“…The LCBD appears to play a role in the subcellular localization of Myo1c in some cell types [73], indicating that light chains may have a role in myosin-I targeting. Myosin-I isoforms from lower eukaryotes co-purify with calmodulin-like proteins (e.g., [74, 75]) rather than calmodulin. Additionally, vertebrate Myo1c has been shown to bind calcium-binding protein 1 (CaBP1) and calcium- and integrin-binding-protein-1 (CIB1) [76].…”

Section: Motor Domain and Lcbd Control Of Localizationmentioning

confidence: 99%

Regulation and control of myosin-I by the motor and light chain-binding domains

Greenberg

Ostap

2013

Trends in Cell Biology

View full text Add to dashboard Cite

Members of the myosin-I family of molecular motors are expressed in many eukaryotes where they are involved in a multitude of critical processes. Humans express 8 distinct members of the myosin-I family, making it the second largest family of myosins expressed in humans. Despite the high degree of sequence conservation in the motor and light chain binding domains of these myosins, recent studies have revealed surprising diversity of function and regulation arising from isoform-specific differences in these domains. Here we review the regulation of myosin-I function and localization by the motor and light chain binding domains.

show abstract

“…Vertebrate Myo1e has a single IQ motif bound by calmodulin that inhibits myosin ATPase activity in the presence of Ca 2+ (24). S. pombe Myo1 has two IQ motifs, IQ1 bound by calmodulin Cam1 and IQ2 bound by the calmodulin-like light chain Cam2 (8,25). The IQ motif of HsMyo1e shares greater amino acid sequence similarity with the first IQ motif of SpMyo1 (38%) than with the second IQ motif (23%) ( Fig.…”

Section: Hsmyo1e Iq Motif Recruits Cam1 But Not Cam2 In S Pombementioning

confidence: 99%

“…Cam2 binding to the lever arm of SpMyo1 has been found to maximize myosin motility in vitro (25). In the absence of Cam2, SpMyo1 still localizes to actin patches, but in the absence of SpMyo1 or when Cam2-IQ2 motif binding is otherwise disrupted, Cam2 moves to larger stationary puncta at the poles as well as mobile cytosolic puncta (25). To determine whether the chimeric proteins were capable of recruiting Cam2, we transformed the mGFP-tagged myosin constructs into a myo1Δ strain expressing Cam2 tagged with mCherry ( Fig.…”

Section: Hsmyo1e Iq Motif Recruits Cam1 But Not Cam2 In S Pombementioning

confidence: 99%

“…Myo1 contains an additional region at the C-terminus of the tail, called the central-acidic domain, which can directly bind the Arp2/3 complex to initiate branched actin nucleation (7,(11)(12)(13)(14). While Myo1e contains a single light-chain binding motif that binds calmodulin (24), S. pombe Myo1 contains two IQ motifs, which bind two distinct light-chain proteins, calmodulin Cam1 and calmodulin-like Cam2 (8,25). Lastly, the motor domains of yeast and mammalian class I myosins differ at the TEDS site, a conserved amino acid residue located on a surface loop within the actin-binding site (26).…”

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Human Myosin 1e tail but not motor domain replaces fission yeast Myo1 domains to support myosin-I function during endocytosis

Barger

James

Pellenz

et al. 2019

Preprint

Self Cite

View full text Add to dashboard Cite

In both unicellular and multicellular organisms, long-tailed class I myosins function in clathrin-mediated endocytosis. Myosin 1e (Myo1e) in vertebrates and Myo1 in fission yeast have similar domain organization, yet whether these proteins or their individual protein domains are functionally interchangeable remains unknown. In an effort to assess functional conservation of class I myosins, we tested whether human Myo1e could replace Myo1 in fission yeast Schizosaccharomyces pombe and found that it was unable to substitute for yeast Myo1. To determine if any individual protein domain is responsible for the inability of Myo1e to function in yeast, we created human-yeast myosin-I chimeras. By functionally testing these chimeric myosins in vivo, we concluded that the Myo1e motor domain is unable to function in yeast, even when combined with the yeast Myo1 tail and a full complement of yeast regulatory light chains. Conversely, the Myo1e tail, when attached to the yeast Myo1 motor domain, supports localization to actin patches and partially rescues the endocytosis defect in myo1Δ cells. Further dissection showed that both the TH1 and TH2-SH3 domains in the human Myo1e tail are required for localization and function of chimeric myosin-I at endocytic sites. Overall, this study provides insights into the role of individual myosin-I domains, expands the utility of fission yeast as a simple model system to study the effects of disease-associated MYO1E mutations, and supports a model of co-evolution between a myosin motor and its actin track.

show abstract

A calmodulin-related light chain from fission yeast that functions with myosin-I and PI 4-kinase

Cited by 18 publications

References 93 publications

Contractile Ring Stability in S. pombe Depends on F-BAR Protein Cdc15p and Bgs1p Transport from the Golgi Complex

Contractile Ring Stability in S. pombe Depends on F-BAR Protein Cdc15p and Bgs1p Transport from the Golgi Complex

Regulation and control of myosin-I by the motor and light chain-binding domains

Human Myosin 1e tail but not motor domain replaces fission yeast Myo1 domains to support myosin-I function during endocytosis

Contact Info

Product

Resources

About