CFP(159-238)-gamma-2 in pcDNAI/Amp
(Plasmid
#55777)
-
PurposeA C-terminal CFP fragment was fused to Ggamma-2. When co-expressed with an N-terminal mCerulean, CFP, or YFP fragment fused to a Gbeta subunit with which it interacts a fluorescent signal is produced.
-
Depositing Lab
-
Sequence Information
Ordering
This material is available to academics and nonprofits only.
| Item | Catalog # | Description | Quantity | Price (USD) | |
|---|---|---|---|---|---|
| Plasmid | 55777 | Standard format: Plasmid sent in bacteria as agar stab | 1 | $85 | |
Backbone
-
Vector backbonepcDNAI/Amp
-
Backbone manufacturerInvitrogen
- Backbone size w/o insert (bp) 4800
- Total vector size (bp) 5242
-
Modifications to backboneA BglII site was introduced into the polylinker of pcDNAI/Amp 3' to the BamHI site.
-
Vector typeMammalian Expression
Growth in Bacteria
-
Bacterial Resistance(s)Ampicillin, 100 μg/mL
-
Growth Temperature37°C
-
Growth Strain(s)DH10B
-
Copy numberHigh Copy
Gene/Insert
-
Gene/Insert nameCFP(159-238)-gamma-2
-
Alt nameGNG2
-
SpeciesH. sapiens (human); Aequorea victoria
-
Insert Size (bp)442
-
MutationCFP(159-238) includes a substitution of His for Asn-164. Ggamma-2 was amplified by PCR, which added a BamHI site and a linker sequence (Arg-Ser) to the 5' end and a 3' BglII site. Cloning into the BglII site of CFP(159-238) destroyed the BamHI site.
-
Entrez GeneGNG2 (a.k.a. HG3F1)
- Promoter CMV
-
Tag
/ Fusion Protein
- CFP(159-238) was fused to the amino terminus of Ggamma-2. (N terminal on insert)
Cloning Information
- Cloning method Restriction Enzyme
- 5′ cloning site BamHI (not destroyed)
- 3′ cloning site BglII (not destroyed)
- 5′ sequencing primer T7
- 3′ sequencing primer SP6 (Common Sequencing Primers)
Resource Information
-
A portion of this plasmid was derived from a plasmid made bypECFP was purchased from Clontech. Gamma-2 cDNA was obtained from Janet Robishaw, Weis Center for Research, Geisinger Clinic, Danville, PA.
Terms and Licenses
-
Academic/Nonprofit Terms
-
Industry Terms
- Not Available to Industry
Trademarks:
- Zeocin® is an InvivoGen trademark.
How to cite this plasmid
( Back to top)
These plasmids were created by your colleagues. Please acknowledge the Principal Investigator, cite the article in which the plasmids were described, and include Addgene in the Materials and Methods of your future publications.
-
For your Materials & Methods section:
CFP(159-238)-gamma-2 in pcDNAI/Amp was a gift from Catherine Berlot (Addgene plasmid # 55777 ; http://n2t.net/addgene:55777 ; RRID:Addgene_55777) -
For your References section:
Live cell analysis of G protein beta5 complex formation, function, and targeting. Yost EA, Mervine SM, Sabo JL, Hynes TR, Berlot CH. Mol Pharmacol. 2007 Oct;72(4):812-25. Epub 2007 Jun 27. 10.1124/mol.107.038075 PubMed 17596375
