Stage-Specific Expression and Targeting of Cyst Wall Protein–Green Fluorescent Protein Chimeras in<i>Giardia</i>

Hehl, Adrian B.; Marti, Matthias; Kohler, Peter O.

doi:10.1091/mbc.11.5.1789

Cited by 98 publications

(147 citation statements)

References 61 publications

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“…To investigate the nature of the fi rst N-terminal hydrophobic sequence, HA tags were introduced at the N-terminal end either of the full-length GlGCS or of a variant lacking the fi rst hydrophobic stretch (aa [3][4][5][6][7][8][9][10][11][12][13][14][15][16][17][18][19][20][21][22]. Both reporters showed an equivalent signal and distribution, indicating that, like the mammalian homolog, the parasite protein is not proteolytically processed to remove the fi rst hydrophobic sequence (data not shown).…”

Section: Discussionmentioning

confidence: 99%

“…New subcultures were obtained by inoculating 5 × 10 4 trophozoites from confl uent cultures into new 11 ml culture tubes. Two-step encystation was induced as described previously ( 19,20 ) by cultivating the cells for ‫ف‬ 44 h in medium without bile (pre-encysting medium) and subsequently in medium with higher pH and porcine bile (encysting medium).…”

Section: Parasite Cell Culturementioning

confidence: 99%

“…All constructs of giardial glucosylceramide synthase (GCS) (GL50803_11642) were based on the expression cassette C1-CWP for inducible expression under the control of the CWP1 promoter ( 19 ). For N-terminal tagging with the hemagglutinin (HA) epitope, full length GCS (aa 2-537) and variant without putative signal peptide (aa 23-537) coding regions were amplifi ed by PCR and cloned in a vector containing the HA epitope tag upstream of the NsiI restriction site.…”

Section: Expression Vector Construction and Transfectionmentioning

confidence: 99%

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Glucosylceramide synthesis inhibition affects cell cycle progression, membrane trafficking, and stage differentiation in Giardia lamblia

Štefanić

Spycher

Morf

et al. 2010

Journal of Lipid Research

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Ceramide, a central molecule in the sphingolipid biosynthesis, plays a critical role as second messenger in cellular signaling that regulates antiproliferative processes, including apoptosis, cell differentiation, and cell cycle arrest in different cell types. Levels of ceramide, a highly bioactive molecule, must be tightly controlled by diverse, coordinated mechanisms, including ceramide degradation, phosphorylation, or sphingolipid metabolism. Glucosylceramide synthase (GCS), also defi ned as ceramide glucosyltransferase (CGT), metabolizes ceramide to glucosylceramide (GlcCer), a glycosylated form of ceramide that does not have antiproliferative activity. GCS plays a crucial role in cell survival after apoptotic stimuli, Abstract Synthesis of glucosylceramide via glucosylceramide synthase (GCS) is a crucial event in higher eukaryotes, both for the production of complex glycosphingolipids and for regulating cellular levels of ceramide, a potent antiproliferative second messenger. In this study, we explored the dependence of the early branching eukaryote Giardia lamblia on GCS activity. Biochemical analyses revealed that the parasite has a GCS located in endoplasmic reticulum (ER) membranes that is active in proliferating and encysting trophozoites. Pharmacological inhibition of GCS induced aberrant cell division, characterized by arrest of cytokinesis, incomplete cleavage furrow formation, and consequent block of replication. Importantly, we showed that increased ceramide levels were responsible for the cytokinesis arrest. In addition, GCS inhibition resulted in prominent ultrastructural abnormalities, including accumulation of cytosolic vesicles, enlarged lysosomes, and clathrin disorganization. Moreover, anterograde traffi cking of the encystations-specifi c protein CWP1 was severely compromised and resulted in inhibition of stage differentiation. Our results reveal novel aspects of lipid metabolism in G. lamblia and specifically highlight the vital role of GCS in regulating cell cycle progression, membrane traffi cking events, and stage differentiation in this parasite. In addition, we identifi ed ceramide as a potent bioactive molecule, underscoring the universal conservation of ceramide signaling in eukaryotes. -Štefanić,

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Section: Discussionmentioning

confidence: 99%

Section: Parasite Cell Culturementioning

confidence: 99%

Section: Expression Vector Construction and Transfectionmentioning

confidence: 99%

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Glucosylceramide synthesis inhibition affects cell cycle progression, membrane trafficking, and stage differentiation in Giardia lamblia

Štefanić

Spycher

Morf

et al. 2010

Journal of Lipid Research

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“…The Giardia endomembrane system undergoes significant morphological changes during stage conversion, culminating in the emergence of large membrane-bound compartments containing cyst wall material (ESVs) and subsequent cyst wall assembly (15)(16)(17). Previous reports have described a Golgi apparatus structure (i.e.…”

Section: A Tem Survey Of the Giardia Membrane Compartment Morphology mentioning

confidence: 99%

An Ancestral Secretory Apparatus in the Protozoan Parasite Giardia intestinalis

Marti

Regös

et al. 2003

Journal of Biological Chemistry

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103

137

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The protozoan parasite Giardia intestinalis belongs to one of the earliest diverged eukaryotic lineages. This is also reflected in a simple intracellular organization, as Giardia lacks common subcellular compartments such as mitochondria, peroxisomes, and apparently also a Golgi apparatus. During encystation, developmentally regulated formation of large secretory compartments containing cyst wall material occurs. Despite the lack of any morphological similarities, these encystation-specific vesicles (ESVs) show several biochemical characteristics of maturing Golgi cisternae. Previous studies suggested that Golgi structure and function are induced only during encystation in Giardia, giving rise to the hypothesis that ESVs, as a Giardia Golgi equivalent, are generated de novo. Alternatively, ESV compartments could be built on the template structure of a cryptic Golgi in trophozoites in response to ER export of cyst wall material during encystation. We addressed this question by defining the molecular framework of the Giardia secretory apparatus using a comparative genomic approach. Analysis of the corresponding transcriptome during growth and encystation revealed surprisingly little stage-specific regulation. A panel of antibodies was generated against selected marker proteins to investigate the developmental dynamics of the endomembrane system. We show evidence that Giardia accommodates the export of large amounts of cyst wall material through re-organization of membrane compartment(s) in trophozoites with biochemical similarities to ESVs. This suggests that ESVs are selectively stabilized Golgi-like compartments in a unique and archetypical secretory system, which arise from a structural template in trophozoites rather than being generated de novo.

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“…It has been shown that 466 bp of the upstream regulatory region of the GL cwp-2 gene is sufficient to control regulated transcription (26). We chose to investigate the transcription of the cwp-2 promoter in a mammalian system because regulation of SREBP is well defined in mammalian cells.…”

Section: Serum-free Medium Induces Cwp-2 Mediated Gene Transcription mentioning

confidence: 99%

Sterol and fatty acid regulatory pathways in a Giardia lamblia-derived promoter

Worgall

Davis-Hayman

Magana

et al. 2004

Journal of Lipid Research

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Giardia lamblia (GL) is a flagellated protozoan that resides in the intestines of different vertebrate hosts. GL is the most frequent cause of waterborne diarrhea worldwide (1). The disease can cause severe malnutrition (2), and infection has been correlated with impaired cognitive development in less-developed countries (3). GL, considered one of the most ancient eukaryotes (4-6), is a diplomonad with a simple life cycle. Infection occurs after the ingestion of cysts contaminating water or food or through person-to-person transmission. Excystation in the duodenum results in the development and release of trophozoites that proliferate in the small intestine. Cysts develop as the trophozoites are swept down the intestine. Importantly, in vitro cholesterol starvation induces trophozoites to differentiate into environmentally resistant cysts (7), a process that occurs in the lower small intestine after the absorption of bile salts and cholesterol. The precise mechanism of cyst wall formation is unknown, but its assembly is preceded by the synthesis, packing, and release of secretory components destined for the cyst wall, such as cyst-wall proteins 1 (CWP-1) and 2 (CWP-2). Upon formation, the cysts are passed in the feces, and the life cycle is completed.The sterol regulatory element binding-proteins (SREBPs) were discovered in mammalian cells (8). SREBPs are pivotal transcription factors of the genes of lipid metabolism. Cholesterol starvation activates a proteolytic cascade that Abbreviations: CHO, Chinese hamster ovary; CWP, cyst wall protein; GL, Giardia lamblia ; mSREBP, mature SREBP; RLU, relative light units; SRE, sterol regulatory element; SREBP, sterol regulatory element binding protein.

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Stage-Specific Expression and Targeting of Cyst Wall Protein–Green Fluorescent Protein Chimeras inGiardia

Cited by 98 publications

References 61 publications

Glucosylceramide synthesis inhibition affects cell cycle progression, membrane trafficking, and stage differentiation in Giardia lamblia

Glucosylceramide synthesis inhibition affects cell cycle progression, membrane trafficking, and stage differentiation in Giardia lamblia

An Ancestral Secretory Apparatus in the Protozoan Parasite Giardia intestinalis

Sterol and fatty acid regulatory pathways in a Giardia lamblia-derived promoter

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