pcmv sport6 vector, by GE Healthcare - Product details

1

Recombinant Expression of AIG1 and ADTRP

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Full-length cDNA encoding human AIG1 (GE Healthcare, in pOTB7 vector) was cloned into the pCMV6-Entry vector with C-terminal Myc and DDK tags. (Sense primer: 5'-GGGCGGCCGGGAATTCGCGAACATGG-3'; Antisense primer: 3'-AAGCCTAAATTGGAAACGCGGCCGCTTTA-5'). Full-length cDNA encoding for human ADTRP in the pCMV6-XL5 vector was purchased from Origene. Full-length cDNA constructs encoding for mouse AIG1 in the pCMV-Sport6 vector, rat AIG1 in pExpress-1 vector, and mouse ADTRP in the pCMV-Sport6 vector were purchased from GE Life Sciences. To recombinantly express AIG1 or ADTRP, HEK293T cells were grown to 40% confluence in a 10 cm tissue culture plate and transiently transfected with 4 μg of the desired construct using polyethyleneimine ‘MAX’ (MW 40,000, PEI; Polysciences, Inc.) as the transfection reagent per the manufacturer’s protocol. ‘Mock’ transfected cells were transfected with 4 μg of empty vector. 48 h after transfection, cells were washed with PBS (3x), harvested by scraping, and lysed by sonication in PBS. The membrane and soluble fractions were separated by ultra-centrifugation at 100,000 g for 45 min at 4 °C. Protein concentrations were measured using the DC Protein Assay kit (Bio-Rad). Aliquots were flash-frozen and stored at −80 °C for further use.

Parsons W.H., Kolar M.J., Kamat S.S., Cognetta AB I.I.I., Hulce J.J., Saez E., Kahn B.B., Saghatelian A, & Cravatt B.F. (2016). AIG1 and ADTRP are Atypical Integral Membrane Hydrolases that Degrade Bioactive FAHFAs. Nature chemical biology, 12(5), 367-372.

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Recombinant Expression of AIG1 and ADTRP

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Full-length cDNA encoding human AIG1 (GE Healthcare, in pOTB7 vector) was cloned into the pCMV6-Entry vector with C-terminal Myc and DDK tags. (Sense primer: 5'-GGGCGGCCGGGAATTCGCGAACATGG-3'; Antisense primer: 3'-AAGCCTAAATTGGAAACGCGGCCGCTTTA-5'). Full-length cDNA encoding for human ADTRP in the pCMV6-XL5 vector was purchased from Origene. Full-length cDNA constructs encoding for mouse AIG1 in the pCMV-Sport6 vector, rat AIG1 in pExpress-1 vector, and mouse ADTRP in the pCMV-Sport6 vector were purchased from GE Life Sciences. To recombinantly express AIG1 or ADTRP, HEK293T cells were grown to 40% confluence in a 10 cm tissue culture plate and transiently transfected with 4 μg of the desired construct using polyethyleneimine ‘MAX’ (MW 40,000, PEI; Polysciences, Inc.) as the transfection reagent per the manufacturer’s protocol. ‘Mock’ transfected cells were transfected with 4 μg of empty vector. 48 h after transfection, cells were washed with PBS (3x), harvested by scraping, and lysed by sonication in PBS. The membrane and soluble fractions were separated by ultra-centrifugation at 100,000 g for 45 min at 4 °C. Protein concentrations were measured using the DC Protein Assay kit (Bio-Rad). Aliquots were flash-frozen and stored at −80 °C for further use.

Parsons W.H., Kolar M.J., Kamat S.S., Cognetta AB I.I.I., Hulce J.J., Saez E., Kahn B.B., Saghatelian A, & Cravatt B.F. (2016). AIG1 and ADTRP are Atypical Integral Membrane Hydrolases that Degrade Bioactive FAHFAs. Nature chemical biology, 12(5), 367-372.

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3

Overexpression of hABHD12 Mutant in HEK293T Cells

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The full-length hABHD12 cDNA was cloned into pCMV-Sport6 vector between NotI and SalI restriction sites (GE Life Sciences). The S246A hABHD12 mutant was generated from the same plasmid using Phusion polymerase and DpnI (New England Biolabs) as per manufacturers instructions. Recombinant WT and S246A hABHD12 was generated from HEK293T cells using established transient transfection protocols32 (link). “Mock” control cells were transfected with an empty vector using the same protocol. The cells were harvested by scraping 48 h after transfection, washed with sterile DPBS (3X), resuspended in 1 mL DPBS, and lysed by sonication. The overexpression of hABHD12 was confirmed by gel-based ABPP and western blot analysis on membrane proteomes of the transfected cells, preparations of which are described earlier.

Kelkar D.S., Ravikumar G., Mehendale N., Singh S., Joshi A., Sharma A.K., Mhetre A., Rajendran A., Chakrapani H, & Kamat S.S. (2019). A Chemical Genetic Screen Identifies ABHD12 as an Oxidized Phosphatidylserine Lipase. Nature chemical biology, 15(2), 169-178.

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Overexpression of hABHD12 Mutant in HEK293T Cells

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The full-length hABHD12 cDNA was cloned into pCMV-Sport6 vector between NotI and SalI restriction sites (GE Life Sciences). The S246A hABHD12 mutant was generated from the same plasmid using Phusion polymerase and DpnI (New England Biolabs) as per manufacturers instructions. Recombinant WT and S246A hABHD12 was generated from HEK293T cells using established transient transfection protocols32 (link). “Mock” control cells were transfected with an empty vector using the same protocol. The cells were harvested by scraping 48 h after transfection, washed with sterile DPBS (3X), resuspended in 1 mL DPBS, and lysed by sonication. The overexpression of hABHD12 was confirmed by gel-based ABPP and western blot analysis on membrane proteomes of the transfected cells, preparations of which are described earlier.

Kelkar D.S., Ravikumar G., Mehendale N., Singh S., Joshi A., Sharma A.K., Mhetre A., Rajendran A., Chakrapani H, & Kamat S.S. (2019). A Chemical Genetic Screen Identifies ABHD12 as an Oxidized Phosphatidylserine Lipase. Nature chemical biology, 15(2), 169-178.

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5

Constructing mfGFP-TRPM7 Pulldown Assays

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The pOG1 vector encoding human TRPM7 was previously described37 (link). Murine hepatocystin in the pCMV-SPORT6 vector (Accession #: BC009816) was from GE Life Sciences (Piscataway, NJ). COOH-terminus FLAG-tagged hepatocystin was cloned into pcDNA5/FRT/TO (Life Technologies, Inc; Grand Island, NY) from the pCMV-SPORT6 vector using primers described in Supplementary Methods file.) To conduct pulldown purification assays we fused fragments of TRPM7′s COOH-terminus to a multifunctional Green Fluorescent Protein (mfGFP) in which GFP was engineered to contain a streptavidin binding peptide (SBP) tag, octa-histidine-tag, and c-Myc-tag in tandem into a loop of GFP38 (link). mfGFP was subcloned into the NheI and HindIII sites of pcDNA6-V5-HisB to make pcDNA6-mfGFP. mfGFP-fusion proteins of TRPM7-COOH terminal fragments were subcloned by PCR into pcDNA6-mfGFP using pcDNA5/FRT/TO-HA-TRPM7 as a template39 (link). The list of primers employed to make the mfGFP constructs are described in the Supplementary Methods file.

Overton J.D., Komiya Y., Mezzacappa C., Nama K., Cai N., Lou L., Fedeles S.V., Habas R, & Runnels L.W. (2015). Hepatocystin is Essential for TRPM7 Function During Early Embryogenesis. Scientific Reports, 5, 18395.

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Pcmv sport6 vector

Lab products found in correlation

5 protocols using pcmv sport6 vector

Recombinant Expression of AIG1 and ADTRP

Recombinant Expression of AIG1 and ADTRP

Overexpression of hABHD12 Mutant in HEK293T Cells

Overexpression of hABHD12 Mutant in HEK293T Cells

Constructing mfGFP-TRPM7 Pulldown Assays

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