Comparison of<i>Schizosaccharomyces pombe</i>expression systems

Forsburg, Susan L.

doi:10.1093/nar/21.12.2955

Cited by 428 publications

(425 citation statements)

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“…Checking by PCR identified a G418-resistant transformant (strain JW46) that had sustained the desired integration event and segregated 2:2 for G418 resistance when crossed to strain 975. In addition, ain1 ϩ was placed under the control of three versions of the thiamine-regulated nmt1 promoter (the wild-type 3nmt1, the attenuated 41nmt1, and the still weaker 81nmt1) (Basi et al, 1993;Forsburg, 1993), with or without an associated NH 2 -terminal GFP tag (Bähler et al, 1998b). The ain1-specific sequences (70 bp) of the forward primer corresponded to nucleotides Ϫ163 to Ϫ94, and those (76 or 70 bp) of the reverse primers corresponded to the complement of the NH 2 -terminal codons.…”

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confidence: 99%

“…To confirm the presence of these introns, the absence of other introns within the fim1 coding region, and the identification of the putative start and stop codons, cDNA sequences were amplified by PCR using the Expand High Fidelity System (Boehringer Mannheim, Indianapolis, IN), one or the other of two cDNA libraries as template, and primers corresponding to fim1 genomic sequences or vector sequences. One library (kindly provided by Dr. C. Albright, Vanderbilt University, Nashville, TN) was constructed in vector pREP3X (Basi et al, 1993;Forsburg, 1993), and the other (Becker et al, 1991) was constructed in vector pDB20. The PCR products were cloned into the pGEM-T Easy vector and sequenced.…”

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Roles of a Fimbrin and an α-Actinin-like Protein in Fission Yeast Cell Polarization and Cytokinesis

Bähler

Pringle

2001

MBoC

143

183

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Eukaryotic cells contain many actin-interacting proteins, including the ␣-actinins and the fimbrins, both of which have actin cross-linking activity in vitro. We report here the identification and characterization of both an ␣-actinin-like protein (Ain1p) and a fimbrin (Fim1p) in the fission yeast Schizosaccharomyces pombe. Ain1p localizes to the actomyosin-containing medial ring in an F-actindependent manner, and the Ain1p ring contracts during cytokinesis. ain1 deletion cells have no obvious defects under normal growth conditions but display severe cytokinesis defects, associated with defects in medial-ring and septum formation, under certain stress conditions. Overexpression of Ain1p also causes cytokinesis defects, and the ain1 deletion shows synthetic effects with other mutations known to affect medial-ring positioning and/or organization. Fim1p localizes both to the cortical actin patches and to the medial ring in an F-actin-dependent manner, and several lines of evidence suggest that Fim1p is involved in polarization of the actin cytoskeleton. Although a fim1 deletion strain has no detectable defect in cytokinesis, overexpression of Fim1p causes a lethal cytokinesis defect associated with a failure to form the medial ring and concentrate actin patches at the cell middle. Moreover, an ain1 fim1 double mutant has a synthetical-lethal defect in medial-ring assembly and cell division. Thus, Ain1p and Fim1p appear to have an overlapping and essential function in fission yeast cytokinesis. In addition, protein-localization and mutant-phenotype data suggest that Fim1p, but not Ain1p, plays important roles in mating and in spore formation. INTRODUCTIONThe actin cytoskeleton is involved in many processes in eukaryotic cells, including the polarization of cell growth and cytokinesis. These many roles involve the interaction of actin with a wide variety of actin-binding proteins, including proteins that can cross-link actin filaments into isotropic gels or bundles. Many actin cross-linking proteins have been purified and studied in vitro, but their functions in vivo remain poorly understood (reviewed by Matsudaira, 1994a;Otto, 1994;Furukawa and Fechheimer, 1997;Ayscough, 1998;Bartles, 2000).Among the actin cross-linking proteins, one of the best characterized is ␣-actinin. It was first isolated from rabbit skeletal muscle (Ebashi and Ebashi, 1965) and has subsequently been identified in both muscle and nonmuscle cells from a variety of animals, in Acanthamoeba, and in Dictyostelium (Furukawa and Fechheimer, 1997;Critchley and Flood, 1999). ␣-Actinin forms a homodimer of antiparallel polypeptides (Critchley and Flood, 1999;Djinovic-Carugo et al., 1999), with the actin-binding domain of each polypeptide close to the NH 2 terminus, followed by four spectrin-like repeats and two COOH-terminal EF-hand motifs. Skeletal muscle isoforms are localized to the Z-disk and are not regulated by Ca 2ϩ , whereas nonmuscle isoforms are localized to focal adhesions, stress fibers, and other structures and are typically regulated by C...

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mentioning

confidence: 99%

mentioning

confidence: 99%

Roles of a Fimbrin and an α-Actinin-like Protein in Fission Yeast Cell Polarization and Cytokinesis

Bähler

Pringle

2001

MBoC

143

183

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“…In the S. cerevisiae complementation test, the Spt4 proteins are expressed from singlecopy CEN plasmids, but no such single-copy plasmid system is available for fission yeast. Instead, we used high-copy vectors that are standard in the field (Forsburg 1993). Therefore, mutations that cause functional deficits at low gene dosage in budding yeast might be missed at high gene dosage in fission yeast, e.g., because increased production of the mutant Spt4 results by mass action in sufficient Spt5-Spt4 complex to support cell growth at 37°C.…”

Section: Deletion Of Spt4 In S Pombementioning

confidence: 99%

“…Therefore, mutations that cause functional deficits at low gene dosage in budding yeast might be missed at high gene dosage in fission yeast, e.g., because increased production of the mutant Spt4 results by mass action in sufficient Spt5-Spt4 complex to support cell growth at 37°C. We attempted to down-regulate transcription of the plasmid-borne nmt1-spt4 + cassette by inclusion of thiamine in the growth medium (Forsburg 1993) and found that the plasmid still complemented growth of the spt4D strain at 37°C (data not shown), implying that Spt4 is indeed produced in functional excess from the high copy plasmid.…”

Section: Deletion Of Spt4 In S Pombementioning

confidence: 99%

“…For expression of Spt4 in fission yeast, DNA fragments encoding wild-type or mutant Spt4 proteins were excised from the respective pYN132-spt4 plasmids and inserted into pREP81x, wherein Spt4 is expressed under the transcriptional control of a weakened nmt1 promoter (Forsburg 1993). Leu + transformants were selected and the growth of the various pREP81x-spt4 strains was compared to spt4D cells that had been transformed with the empty pREP81x plasmid.…”

Section: Deletion Of Spt4 In S Pombementioning

confidence: 99%

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Characterization of the Schizosaccharomyces pombe Spt5-Spt4 complex

Schwer

Schneider²,

Pei³

et al. 2009

RNA

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The Spt5-Spt4 complex regulates early transcription elongation by RNA polymerase II and has an imputed role in pre-mRNA processing via its physical association with mRNA capping enzymes. Here we characterize the Schizosaccharomyces pombe core Spt5-Spt4 complex as a heterodimer and map a trypsin-resistant Spt4-binding domain within the Spt5 subunit. A genetic analysis of Spt4 in S. pombe revealed it to be inessential for growth at 25°C-30°C but critical at 37°C. These results echo the conditional spt4D growth phenotype in budding yeast, where we find that Saccharomyces cerevisiae and S. pombe Spt4 are functionally interchangeable. Complementation of S. cerevisiae spt4D and a two-hybrid assay for Spt4-Spt5 interaction provided a readout of the effects of 33 missense and truncation mutations on S. pombe Spt4 function in vivo, which were interpreted in light of the recent crystal structure of S. cerevisiae Spt4 fused to a fragment of Spt5. Our results highlight the importance of the Spt4 Zn 2+ -binding residues-Cys12, Cys15, Cys29, and Asp32-and of Ser57, a conserved constituent of the Spt4-Spt5 interface. The 990-amino acid S. pombe Spt5 protein has an exceptionally regular carboxyl-terminal domain (CTD) composed of 18 nonapeptide repeats. We find that as few as three nonamer repeats sufficed for S. pombe growth, but only when Spt4 was present. Synthetic lethality of the spt5 1-835 spt4D double mutant at 34°C suggests that interaction of Spt4 with the central domain of Spt5 overlaps functionally with the Spt5 CTD.

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Molecular, functional and evolutionary characterization of the gene encoding HMG-CoA reductase in the fission yeast,Schizosaccharomyces pombe

Lum

Edwards

Wright

1996

Yeast

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The synthesis of mevalonate, a molecule required for both sterol and isoprene biosynthesis in eukaryotes, is catalysed by 3‐hydroxy‐3‐methylglutaryl coenzyme A (HMG‐CoA) reductase. Using a gene dosage approach, we have isolated the gene encoding HMG‐CoA reductase, hmg1+, from the fission yeast Schizosaccharomyces pombe (Accession Number L76979). Specifically, hmg1+ was isolated on the basis of its ability to confer resistance to lovastatin, a competitive inhibitor of HMG‐CoA reductase. Gene disruption analysis showed that hmg1+ was an essential gene. This result provided evidence that, unlike Saccharomyces cerevisiae, S. pombe contained only a single functional HMG‐CoA reductase gene. The presence of a single HMG‐CoA reductase gene was confirmed by genomic hybridization analysis. As observed for the S. cerevisiae HMG1p, the hmg1+ protein induced membrane proliferations known as karmellae. A previously undescribed ‘feed‐forward’ regulation was observed in which elevated levels of HMG‐CoA synthase, the enzyme catalysing the synthesis of the HMG‐CoA reductase substrate, induced elevated levels of hmg1+ protein in the cell and conferred partial resistance to lovastatin. The amino acid sequences of yeast and human HMG‐CoA reductase were highly divergent in the membrane domains, but were extensively conserved in the catalytic domains. We tested whether the gene duplication that produced the two functional genes in S. cerevisiae occurred before or after S. pombe and S. cerevisiae diverged by comparing the log likelihoods of trees specified by these hypotheses. We found that the tree specifying post‐divergence duplication had significantly higher likelihood. Moreover, phylogenetic analyses of available HMG‐CoA reductase sequences also suggested that the lineages of S. pombe and S. cerevisiae diverged approximately 420 million years ago but that the duplication event that produced two HMG‐CoA reductase genes in the budding yeast occurred only approximately 56 million years ago. To date, S. pombe is the only unicellular eukaryote that has been found to contain a single HMG‐CoA reductase gene. Consequently, S. pombe may provide important opportunities to study aspects of the regulation of sterol biosynthesis that have been difficult to address in other organisms and serve as a test organism to identify novel therapies for modulating cholesterol synthesis.

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Comparison ofSchizosaccharomyces pombeexpression systems

Cited by 428 publications

References 7 publications

Roles of a Fimbrin and an α-Actinin-like Protein in Fission Yeast Cell Polarization and Cytokinesis

Roles of a Fimbrin and an α-Actinin-like Protein in Fission Yeast Cell Polarization and Cytokinesis

Characterization of the Schizosaccharomyces pombe Spt5-Spt4 complex

Molecular, functional and evolutionary characterization of the gene encoding HMG-CoA reductase in the fission yeast,Schizosaccharomyces pombe

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