ProQuest™ Two-Hybrid System with Gateway™ Technology

Name: ProQuest™ Two-Hybrid System with Gateway™ Technology
SKU: PQ1000101
Price: 1728.00 USD

The ProQuest™ Two-Hybrid System with Gateway™ Technology is an in vivo yeast-based system for identifying interactions between two proteins. ThisRead more

Catalog number PQ1000101

Price (USD)

1,728.00

Each

Add to cart

Price (USD)

1,728.00

Each

Add to cart

The ProQuest™ Two-Hybrid System with Gateway™ Technology is an in vivo yeast-based system for identifying interactions between two proteins. This interaction reconstitutes a functional transcription factor that activates chromosomally integrated reporter genes where transcriptional activation is monitored by the growth of cells on selective media.
The ProQuest™ System features:
• Gateway™ Technology to allow rapid and easy generation of bait and prey constructs, and to facilitate downstream application
• Low copy-number DBD (DNA Binding Domain) and AD (Activation Domain) vectors (ARS/CEN) to control over-expression and increase reproducibility
• Three different reporter genes (HIS3, URA3, and lacZ) with independent promoter regions to rapidly weed out false positives. URA3 reporter gene allows for both positive and negative selection, enabling advanced two-hybrid techniques such as reverse two-hybrid.

• A set of strong-to-weak Gateway™-based control interactions to evaluate results and assess the strength of the interaction being tested

For Research Use Only. Not for use in diagnostic procedures.

Specifications

Product TypeTwo-Hybrid System

Reporter GeneBeta-Gal (lacZ), HIS3, URA3

AssayTwo-Hybrid Assay

Expression SystemYeast

Quantity1 kit

Product LineGateway™, ProQuest™

Unit SizeEach

Contents & Storage

The ProQuest™ Two-Hybrid System includes yeast expression vectors pDEST™32, pDEST™22, and pEXP-AD502 for generation of GAL4 DNA Binding Domain and GAL4 Activation Domain fusion proteins, and LR Clonase™ II Enzyme Mix, a glycerol stock of the MaV203 yeast strain, as well as positive and negative controls for the two-hybrid assay. Store kit components at -80°C. Guaranteed stable for six months when properly stored.

Frequently asked questions (FAQs)

How large of a PCR product can I recombine with a pDONR vector via BP cloning? Does the same apply for TOPO-adapted Entry vectors?

There is no theoretical limit to insert size for a BP reaction with a pDONR vector. Maximum size tested in-house is 12 kb. TOPO vectors are more sensitive to insert size and 3-5 kb is the upper limit for decent cloning efficiency.

How should I clean up my attB-PCR product?

After generating your attB-PCR product, we recommend purifying it to remove PCR buffer, unincorporated dNTPs, attB primers, and any attB primer-dimers. Primers and primer-dimers can recombine efficiently with the Donor vector in the BP reaction and may increase background after transformation into E. coli, whereas leftover PCR buffer may inhibit the BP reaction. Standard PCR product purification protocols using phenol/chloroform extraction followed by ammonium acetate and ethanol or isopropanol precipitation are not recommended for purification of the attB-PCR product as these protocols generally have exclusion limits of less than 100 bp and do not efficiently remove large primer-dimer products. We recommend a PEG purification protocol (see page 17 of the Gateway Technology with Clonase II manual). If you use the above protocol and your attB-PCR product is still not suitably purified, you may further gel-purify the product. We recommend using the PureLink Quick Gel Extraction kit.

I'm trying to propagate my Gateway destination vector and am not seeing any colonies. What should I do?

Check the genotype of the cell strain you are using. Our Gateway destination vectors typically contain a ccdB cassette, which, if uninterrupted, will inhibit E. coli growth. Therefore, un-cloned vectors should be propagated in a ccdB survival cell strain, such as our ccdB Survival 2 T1R competent cells.

Why does my prestained standard give different molecular weights for different types of gels?

Protein gels vary in pH. Each of the proteins in the standard has a dye molecule attached to it, and the charge on these dye molecules can change depending on the pH of the gel. This change in charge will affect the migration of the protein on the gel.

Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.

Is the ProQuest Two-Hybrid System suitable for protein-protein interaction studies with membrane proteins?

The ProQuest Two-Hybrid System is not suitable for proteins containing membrane spanning domains. Protein interaction and activation of transcription of the reporter genes depends on the proteins localizing to the nucleus. You can remove membrane-spanning regions or include only cytosolic or extracelluar domains of membrane bound protein in the bait or prey constructs.

Find additional tips, troubleshooting help, and resources within our Protein Assays and Analysis Support Center.

View all ProQuest™ Two-Hybrid System with Gateway™ Technology FAQs