Your search keyword '"Castillon GA"' showing total 7 results

1. An essential function of sphingolipids in yeast cell division.

Author

Epstein S, Castillon GA, Qin Y, and Riezman H

Subjects

Gene Deletion, Gossypium enzymology, Gossypium genetics, Hexosyltransferases genetics, Metabolic Engineering, Metabolic Networks and Pathways genetics, Microbial Viability, Models, Biological, Molecular Sequence Data, Oxidoreductases genetics, Oxidoreductases metabolism, Recombinant Proteins genetics, Recombinant Proteins metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae metabolism, Sequence Analysis, DNA, Cell Division, Ceramides metabolism, Hexosyltransferases metabolism, Saccharomyces cerevisiae physiology

Abstract

Ceramides are bioactive lipids and precursors to sphingolipids. They have been shown to take part in a wide variety of different physiological processes in eukaryotic organisms and are thought to be toxic at high concentrations. Ceramide is synthesized by condensation of the sphingoid base sphinganine and a fatty acyl CoA by ceramide synthases, a family of enzymes that differ in their specificity for the length of the acyl CoA substrate. We have engineered a yeast strain where the endogenous ceramide synthase has been replaced by one of the putative enzymes from cotton. As a result, the yeast strain produces C18 rather than C26 ceramides showing that the cotton protein is a bona fide ceramide synthase with specificity towards C18 acyl CoA. Strikingly, the accumulation of C18 ceramide is not toxic in Saccharomyces cerevisiae. This allows survival of the yeast after deletion of the normally essential AUR1 (inositol phosphorylceramide synthase) gene permitting us to address the essential roles of sphingolipids. Deletion of AUR1 allows cell growth, but leads to a defect in cytokinesis, which takes twice as long as in wild-type strains. Nuclear division and recruitment of septins is apparently not affected, but cytokinesis is delayed and cell separation is incomplete., (© 2012 Blackwell Publishing Ltd.)

Published

2012

2. Activation of the unfolded protein response pathway causes ceramide accumulation in yeast and INS-1E insulinoma cells.

Author

Epstein S, Kirkpatrick CL, Castillon GA, Muñiz M, Riezman I, David FPA, Wollheim CB, and Riezman H

Subjects

Animals, Cell Line, Tumor, Endoplasmic Reticulum Stress genetics, Endoplasmic Reticulum Stress physiology, Oxidoreductases genetics, Oxidoreductases metabolism, Rats, Reverse Transcriptase Polymerase Chain Reaction, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins genetics, Saccharomyces cerevisiae Proteins metabolism, Spectrometry, Mass, Electrospray Ionization, Sphingomyelins metabolism, Unfolded Protein Response genetics, Vesicular Transport Proteins genetics, Vesicular Transport Proteins metabolism, Ceramides metabolism, Insulinoma metabolism, Saccharomyces cerevisiae metabolism, Unfolded Protein Response physiology

Abstract

Sphingolipids are not only important components of membranes but also have functions in protein trafficking and intracellular signaling. The LCB1 gene encodes a subunit of the serine palmitoyltransferase, which is responsible for the first step of sphingolipid synthesis. Here, we show that activation of the unfolded protein response (UPR) can restore normal ceramide levels and viability in yeast cells with a conditional defect in LCB1. Dependence on UPR was demonstrated by showing the HAC1-dependence of the suppression. A similar induction of ceramides by UPR seems to take place in mammalian cells. In rat pancreatic INS-1E cells, UPR activation induces the transcription of the CerS6 gene, which encodes a ceramide synthase. This correlates with the specific accumulation of ceramide with a C16 fatty acyl chain upon UPR activation. Therefore, our study reveals a novel connection between UPR induction and ceramide synthesis that seems to be conserved between yeast and mammalian cells.

Published

2012

3. The yeast p24 complex regulates GPI-anchored protein transport and quality control by monitoring anchor remodeling.

Author

Castillon GA, Aguilera-Romero A, Manzano-Lopez J, Epstein S, Kajiwara K, Funato K, Watanabe R, Riezman H, and Muñiz M

Subjects

Binding Sites, Endoplasmic Reticulum metabolism, Endoplasmic Reticulum Stress, Gene Knockout Techniques, Golgi Apparatus metabolism, Membrane Proteins metabolism, Multiprotein Complexes chemistry, Multiprotein Complexes genetics, Protein Binding, Protein Transport, Saccharomyces cerevisiae Proteins chemistry, Saccharomyces cerevisiae Proteins genetics, Unfolded Protein Response, Vesicular Transport Proteins chemistry, Vesicular Transport Proteins genetics, GPI-Linked Proteins metabolism, Glycosylphosphatidylinositols metabolism, Multiprotein Complexes metabolism, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism, Vesicular Transport Proteins metabolism

Abstract

Glycosylphosphatidylinositol (GPI)-anchored proteins are secretory proteins that are attached to the cell surface of eukaryotic cells by a glycolipid moiety. Once GPI anchoring has occurred in the lumen of the endoplasmic reticulum (ER), the structure of the lipid part on the GPI anchor undergoes a remodeling process prior to ER exit. In this study, we provide evidence suggesting that the yeast p24 complex, through binding specifically to GPI-anchored proteins in an anchor-dependent manner, plays a dual role in their selective trafficking. First, the p24 complex promotes efficient ER exit of remodeled GPI-anchored proteins after concentration by connecting them with the COPII coat and thus facilitates their incorporation into vesicles. Second, it retrieves escaped, unremodeled GPI-anchored proteins from the Golgi to the ER in COPI vesicles. Therefore the p24 complex, by sensing the status of the GPI anchor, regulates GPI-anchored protein intracellular transport and coordinates this with correct anchor remodeling.

Published

2011

4. Functional interactions between sphingolipids and sterols in biological membranes regulating cell physiology.

Author

Guan XL, Souza CM, Pichler H, Dewhurst G, Schaad O, Kajiwara K, Wakabayashi H, Ivanova T, Castillon GA, Piccolis M, Abe F, Loewith R, Funato K, Wenk MR, and Riezman H

Subjects

Anisotropy, Biological Transport drug effects, Caffeine pharmacology, Cell Membrane drug effects, Cluster Analysis, Gene Expression Profiling, Mutation genetics, Phenotype, Saccharomyces cerevisiae drug effects, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins metabolism, Sirolimus pharmacology, Sorbic Acid pharmacology, Sphingolipids chemistry, Sterols biosynthesis, Sterols chemistry, Cell Membrane physiology, Saccharomyces cerevisiae cytology, Saccharomyces cerevisiae physiology, Sphingolipids metabolism, Sterols metabolism

Abstract

Sterols and sphingolipids are limited to eukaryotic cells, and their interaction has been proposed to favor formation of lipid microdomains. Although there is abundant biophysical evidence demonstrating their interaction in simple systems, convincing evidence is lacking to show that they function together in cells. Using lipid analysis by mass spectrometry and a genetic approach on mutants in sterol metabolism, we show that cells adjust their membrane composition in response to mutant sterol structures preferentially by changing their sphingolipid composition. Systematic combination of mutations in sterol biosynthesis with mutants in sphingolipid hydroxylation and head group turnover give a large number of synthetic and suppression phenotypes. Our unbiased approach provides compelling evidence that sterols and sphingolipids function together in cells. We were not able to correlate any cellular phenotype we measured with plasma membrane fluidity as measured using fluorescence anisotropy. This questions whether the increase in liquid order phases that can be induced by sterol-sphingolipid interactions plays an important role in cells. Our data revealing that cells have a mechanism to sense the quality of their membrane sterol composition has led us to suggest that proteins might recognize sterol-sphingolipid complexes and to hypothesize the coevolution of sterols and sphingolipids.

Published

2009

5. Concentration of GPI-anchored proteins upon ER exit in yeast.

Author

Castillon GA, Watanabe R, Taylor M, Schwabe TM, and Riezman H

Subjects

Amino Acid Transport Systems genetics, Amino Acid Transport Systems metabolism, Cell Wall genetics, Cytoplasmic Vesicles metabolism, Glucose Transport Proteins, Facilitative, Membrane Glycoproteins genetics, Membrane Proteins genetics, Membrane Proteins metabolism, Monosaccharide Transport Proteins genetics, Monosaccharide Transport Proteins metabolism, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins genetics, Temperature, Vesicular Transport Proteins genetics, Vesicular Transport Proteins metabolism, Cell Wall metabolism, Endoplasmic Reticulum metabolism, Glycosylphosphatidylinositols metabolism, Membrane Glycoproteins metabolism, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism

Abstract

Previous biochemical work has revealed two parallel routes of exit from the endoplasmic reticulum (ER) in the yeast Saccharomyces cerevisiae, one seemingly specific for glycosyl-phosphatidylinositol (GPI)-anchored proteins. Using the coat protein II (COPII) mutant sec31-1, we visualized ER exit sites (ERES) and identified three distinct ERES populations in vivo. One contains glycosylated pro-alpha-factor, the second contains the GPI-anchored proteins Cwp2p, Ccw14p and Tos6p and the third is enriched with the hexose transporter, Hxt1p. Concentration of GPI-anchored proteins prior to budding requires anchor remodeling, and Hxt1p incorporation into ERES requires the COPII components Sec12p and Sec16p. Additionally, we have found that GPI-anchored protein ER exit is controlled by the p24 family member Emp24p, whereas ER export of most transmembrane proteins requires the Cornichon homologue Erv14p.

Published

2009

6. The presence of an ER exit signal determines the protein sorting upon ER exit in yeast.

Author

Watanabe R, Castillon GA, Meury A, and Riezman H

Subjects

Amino Acid Transport Systems chemistry, Amino Acid Transport Systems genetics, Amino Acid Transport Systems metabolism, Golgi Apparatus metabolism, Immunoprecipitation, Open Reading Frames, Protein Binding, Protein Precursors genetics, Protein Precursors metabolism, Protein Transport, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins chemistry, Saccharomyces cerevisiae Proteins genetics, Vesicular Transport Proteins chemistry, Vesicular Transport Proteins genetics, Vesicular Transport Proteins metabolism, Endoplasmic Reticulum metabolism, Saccharomyces cerevisiae metabolism, Saccharomyces cerevisiae Proteins metabolism

Abstract

In yeast, there are at least two vesicle populations upon ER (endoplasmic reticulum) exit, one containing Gap1p (general aminoacid permease) and a glycosylated alpha-factor, gpalphaF (glycosylated proalpha-factor), and the other containing GPI (glycosylphosphatidylinositol)-anchored proteins, Gas1p (glycophospholipid-anchored surface protein) and Yps1p. We attempted to identify sorting determinants for this protein sorting event in the ER. We found that mutant Gas1 proteins that lack a GPI anchor and/or S/T region (serine- and threonine-rich region), two common characteristic features conserved among yeast GPI-anchored proteins, were still sorted away from Gap1p-containing vesicles. Furthermore, a mutant glycosylated alpha-factor, gpalphaGPI, which contains both the GPI anchor and S/T region from Gas1p, still entered Gap1p-containing vesicles, demonstrating that these conserved characteristics do not prevent proteins from entering Gap1p-containing vesicles. gpalphaF showed severely reduced budding efficiency in the absence of its ER exit receptor Erv29p, and this residual budding product no longer entered Gap1p-containing vesicles. These results suggest that the interaction of gpalphaF with Erv29p is essential for sorting into Gap1p-containing vesicles. We compared the detergent solubility of Gas1p and the gpalphaGPI in the ER with that in ER-derived vesicles. Both GPI-anchored proteins similarly partitioned into the DRM (detergent-resistant membrane) in the ER. Based on the fact that they entered different ER-derived vesicles, we conclude that DRM partitioning of GPI-anchored proteins is not the dominant determinant of protein sorting upon ER exit. Interestingly, upon incorporation into the ER-derived vesicles, gpalphaGPI was no longer detergent-insoluble, in contrast with the persistent detergent insolubility of Gas1p in the ER-derived vesicles. We present different explanations for the different behaviours of GPI-anchored proteins in distinct ER-derived vesicle populations.

Published

2008

7. Septins have a dual role in controlling mitotic exit in budding yeast.

Author

Castillon GA, Adames NR, Rosello CH, Seidel HS, Longtine MS, Cooper JA, and Heil-Chapdelaine RA

Subjects

Cytoskeletal Proteins metabolism, Guanine Nucleotide Exchange Factors metabolism, Microscopy, Fluorescence, Monomeric GTP-Binding Proteins metabolism, Mutation genetics, Saccharomyces cerevisiae genetics, Saccharomyces cerevisiae Proteins metabolism, Cell Cycle Proteins metabolism, Cytoskeletal Proteins physiology, Mitosis physiology, Mutation physiology, Saccharomyces cerevisiae cytology, Spindle Apparatus physiology

Abstract

In Saccharomyces cerevisiae, the spindle position checkpoint ensures that cells do not exit mitosis until the mitotic spindle moves into the mother/bud neck and thus guarantees that each cell receives one nucleus [1-6]. Mitotic exit is controlled by the small G protein Tem1p. Tem1p and its GTPase activating protein (GAP) Bub2p/Bfa1p are located on the daughter-bound spindle pole body. The GEF Lte1p is located in the bud. This segregation helps keep Tem1p in its inactive GDP state until the spindle enters the neck. However, the checkpoint functions without Lte1p and apparently senses cytoplasmic microtubules in the mother/bud neck [7-9]. To investigate this mechanism, we examined mutants defective for septins, which compose a ring at the neck [10]. We found that the septin mutants sep7Delta and cdc10Delta are defective in the checkpoint. When movement of the spindle into the neck was delayed, mitotic exit occurred, inappropriately leaving both nuclei in the mother. In sep7Delta and cdc10Delta mutants, Lte1p is mislocalized to the mother. In sep7Delta, but not cdc10Delta, mutants, inappropriate mitotic exit depends on Lte1p. These results suggest that septins serve as a diffusion barrier for Lte1p, and that Cdc10p is needed for the septin ring to serve as a scaffold for a putative microtubule sensor.

Published

2003