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  • Matchmaker Gold Yeast Two-Hybrid System
  • Yeast two-hybrid libraries
  • Yeast two-hybrid library construction
  • Yeast two-hybrid vectors
  • Yeast strains
  • Prey rescue by colony PCR
Home › Products › Protein research › Two-hybrid and one-hybrid systems › Yeast two-hybrid system › Yeast two-hybrid library construction

Two-hybrid and one-hybrid systems

  • Yeast two-hybrid system
    • Matchmaker Gold Yeast Two-Hybrid System
    • Yeast two-hybrid libraries
      • Normalized Mate & Plate Libraries
    • Yeast two-hybrid library construction
    • Yeast two-hybrid vectors
    • Yeast strains
    • Prey rescue by colony PCR
  • Yeast media
    • Aureobasidin A
    • Yeast two-hybrid media
    • Yeast one-hybrid media
    • Minimal media pouches (ready-mixed)
    • YPDA rich media
    • SD base
    • Amino acid dropout mixes
    • X-alpha-Gal
  • Yeast transformation kits
    • Yeastmaker transformation system
    • Quick & Easy Yeast Transformation Mix
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Yeast two-hybrid library construction

Our convenient "Mate & Plate” libraries eliminate the time-consuming and labor-intensive cloning and amplification steps required in traditional two-hybrid library manufacturing and screening. These ready-to-go libraries require only simple co-culturing of the MATalpha library strain with your bait-expressing reporter strain (MATa), followed by selection on appropriate minimal medium.

Our convenient "Mate & Plate” libraries eliminate the time-consuming and labor-intensive cloning and amplification steps required in traditional two-hybrid library manufacturing and screening. These ready-to-go libraries require only simple co-culturing of the MATalpha library strain with your bait-expressing reporter strain (MATa), followed by selection on appropriate minimal medium.

Do it yourself, simply and quickly

If our selection of ready-made libraries does not suit your needs, you may wish to Make Your Own Mate & Plate Library just the way we do it. Our system provides the materials and methods you need to create enough library vials for hundreds of yeast two-hybrid screens—in less than a week.

Library creation occurs directly in our Y187 library yeast stain, utilizing the highly efficient homologous recombination machinery of Saccharomyces cerevisiae. There is no need for the labor-intensive library cloning, amplification, and harvesting steps that are required by traditional methods of library construction.

Sensitivity

The system uses SMART cDNA synthesis technology, which allows you to construct cDNA libraries from any tissue source starting with as little as 100 ng of total RNA.

What is SMART technology?

Our SMART technology is based on two specific features of Moloney murine leukemia virus reverse transcriptase (MMLV RT):

  • Terminal-transferase activity
  • Template-switching activity

First-strand cDNA synthesis is primed by a modified oligo(dT) primer or random primers. When the MMLV RT reaches the 5’ end of the mRNA, the enzyme’s terminal transferase activity attaches non-template-directed nucleotides onto the newly synthesized strand of cDNA. Then the chemically modified SMART oligo pairs with the extended tail, and serves as a second template onto which the RT enzyme switches to complete first-strand synthesis.

SMART cDNA synthesis ultimately results in cDNA that contains known universal primer binding sequences at either end. As a result, SMART first-strand cDNA is:

  • Available for PCR amplification, enabling you to start from nanogram amounts of RNA, so you can make a library from microdissected tissues, laser-captured cells, biopsy samples, etc.
  • Homologous to the ends of the Matchmaker Gold prey plasmid, pGADT7-Rec; the library is created by cotransforming the yeast strain Y187 with pGADT7-Rec and the SMART cDNA.
 More  Less
Cat. # Product Size Price License Quantity Details
630490 Make Your Own "Mate & Plate™" Library System 5 Rxns USD $1786.00

Mate & Plate Libraries are by far the easiest libraries to screen for protein-protein interactions using a GAL4 yeast two-hybrid system. Several Mate & Plate Libraries are available ready-made from Takara Bio. For libraries that are not available, this system provides the necessary components and a simple, highly efficient method to make your own Mate & Plate Library using SMART technology and the highly efficient homologous recombination machinery of Saccharomyces cerevisiae.

Notice to purchaser

Our products are to be used for Research Use Only. They may not be used for any other purpose, including, but not limited to, use in humans, therapeutic or diagnostic use, or commercial use of any kind. Our products may not be transferred to third parties, resold, modified for resale, or used to manufacture commercial products or to provide a service to third parties without our prior written approval.

Documents Components Image Data

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Library generation using n vivo recombination in S. cerevisiae. Mate & Plate Libraries are created via recombination between your cDNA and the Matchmaker prey vector pGADT7-Rec.

 Library generation using n vivo recombination in S. cerevisiae. Mate & Plate Libraries are created via recombination between your cDNA and the Matchmaker prey vector pGADT7-Rec.
Library generation using in vivo recombination in S. cerevisiae. Mate & Plate Libraries are created via recombination between your cDNA and the Matchmaker prey vector pGADT7-Rec. The homologues are generated by SMART cDNA synthesis. Colonies are pooled, mixed, and aliquoted into multiple vials. Each single 1 ml vial can be used for a two-hybrid screen.

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Mate & Plate libraries display broad insert representation

Mate & Plate libraries display broad insert representation
Mate & Plate libraries display broad insert representation. A human bone marrow library was made using the Make Your Own “Mate & Plate” Library System. Inserts from 15 randomly picked colonies were analyzed by yeast colony PCR using the Advantage 2 Polymerase Mix (Cat. No. 639201), and the Matchmaker AD LD-Insert Screening Amplimer Set (Cat. No. 630433). As seen in Lanes 1–15, every colony contained an insert of a different size. Lane M: 1 kb DNA ladder molecular weight marker.

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SMART cDNA synthesis generates cDNA ends with homology to pGADT7-Rec

SMART cDNA synthesis generates cDNA ends with homology to pGADT7-Rec
SMART cDNA synthesis generates cDNA ends with homology to pGADT7-Rec.

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630490: Make Your Own "Mate & Plate" Library System

630490: Make Your Own "Mate & Plate" Library System

Required Products

Cat. # Product Size Price License Quantity Details
639206 Advantage® 2 PCR Kit 100 Rxns USD $580.00

This kit is based on Takara's Advantage 2 Polymerase Mix. It contains all reagents needed for a hot-start PCR, including control template and primer mix. This kit is ideal for PCR applications that require high fidelity, such as cDNA amplification or library construction. Enough reagents are supplied for 100 PCR reactions of 50 μl each.

Documents Components Image Data

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639206: Advantage 2 PCR Kit

639206: Advantage 2 PCR Kit

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Amplification of a fragment of the rare tumor necrosis factor receptor II (TNFR II) cDNA with Advantage 2 Polymerase Mix and a competitor's Taq polymerase mix

Amplification of a fragment of the rare tumor necrosis factor receptor II (TNFR II) cDNA with Advantage 2 Polymerase Mix and a competitor's Taq polymerase mix
Amplification of a fragment of the rare tumor necrosis factor receptor II (TNFR II) cDNA with Advantage 2 Polymerase Mix and a competitor's Taq polymerase mix. 5 μl of PCR products were run on a 1.1% agarose/EtBr gel. Lane 1: The 0.4-kb TNFR II fragment is readily obtained with Advantage 2. Lane 2: No product is seen with Taq polymerase. Lane M: DNA size marker

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Amplification of various large templates using Advantage 2 Polymerase Mix

Amplification of various large templates using Advantage 2 Polymerase Mix
Amplification of various large templates using Advantage 2 Polymerase Mix. 1–3 μl of each PCR product was run on a 1.1% agarose/EtBr gel. Lane 1: 2.5-kb E. coli DNA polymerase gene amplified from genomic DNA. Lane 2: 3.5-kb bovine pancreatic trypsin inhibitor gene amplified from calf thymus genomic DNA. Lane 3: 5.9-kb human IL-1β gene amplified from human genomic DNA. Lane 4: 8.5-kb human titin cDNA amplified from a SMART Human Skeletal Muscle cDNA library. Lane 5: 18.5-kb λ insert amplified from a λ clone. Lane M: λ/Hind III DNA size marker.
630489 Matchmaker® Gold Yeast Two-Hybrid System Each USD $1180.00

Complete GAL4-based two-hybrid system to detect protein interactions. Yeast strain Y2HGold facilitates the elimination of many false positives that arise when screening an activation domain (AD) fusion library, because it contains four separate reporter genes that can be used to select for protein interactions. The system is also characterized by low background due to the Aureobasidin A resistance marker.

Documents Components You May Also Like Image Data

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The yeast two-hybrid principle

The yeast two-hybrid principle
The yeast two-hybrid principle. A bait protein interacts with the GAL4 recognition sequence (or promoter) upstream of a reporter gene. Transcription of the reporter is activated when a prey protein containing the GAL4 transcriptional activation domain interacts with the bait.

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Matchmaker Gold reporter genes

Matchmaker Gold reporter genes
Matchmaker Gold reporter genes. Yeast strain Y2HGold expresses 4 genes from 3 separate GAL4-responsive promoters in response to protein-protein interactions.

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Four reporters give the Matchmaker Gold Yeast Two-Hybrid System its high stringency

Four reporters give the Matchmaker Gold Yeast Two-Hybrid System its high stringency
Four reporters give the Matchmaker Gold Yeast Two-Hybrid System its high stringency. Interacting bait and prey fusion proteins drive the expression of four different reporters from three different GAL4-responsive promoters (M1, G1, and G2), which are stably integrated in the genome of the reporter strain, Y2H Gold. Aureobasidin A (AbA) resistance and the two auxotrophic reporters for histidine and adenine biosynthesis confer growth selection in the presence of AbA and on histidine- and adenine-deficient media, while the a-galactosidase reporter produces blue colonies in the presence of X-alpha-Gal.

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630489: Matchmaker Gold Yeast Two-Hybrid System

630489: Matchmaker Gold Yeast Two-Hybrid System
639207 Advantage® 2 PCR Kit 30 Rxns USD $188.00

This kit is based on Takara's Advantage 2 Polymerase Mix. It contains all reagents needed for a hot-start PCR, including control template and primer mix. This kit is ideal for PCR applications that require high fidelity, such as cDNA amplification or library construction. Enough reagents are supplied for 30 PCR reactions of 50 μl each.

Documents Components Image Data

Back

Amplification of a fragment of the rare tumor necrosis factor receptor II (TNFR II) cDNA with Advantage 2 Polymerase Mix and a competitor's Taq polymerase mix

Amplification of a fragment of the rare tumor necrosis factor receptor II (TNFR II) cDNA with Advantage 2 Polymerase Mix and a competitor's Taq polymerase mix
Amplification of a fragment of the rare tumor necrosis factor receptor II (TNFR II) cDNA with Advantage 2 Polymerase Mix and a competitor's Taq polymerase mix. 5 μl of PCR products were run on a 1.1% agarose/EtBr gel. Lane 1: The 0.4-kb TNFR II fragment is readily obtained with Advantage 2. Lane 2: No product is seen with Taq polymerase. Lane M: DNA size marker

Back

Amplification of various large templates using Advantage 2 Polymerase Mix

Amplification of various large templates using Advantage 2 Polymerase Mix
Amplification of various large templates using Advantage 2 Polymerase Mix. 1–3 μl of each PCR product was run on a 1.1% agarose/EtBr gel. Lane 1: 2.5-kb E. coli DNA polymerase gene amplified from genomic DNA. Lane 2: 3.5-kb bovine pancreatic trypsin inhibitor gene amplified from calf thymus genomic DNA. Lane 3: 5.9-kb human IL-1β gene amplified from human genomic DNA. Lane 4: 8.5-kb human titin cDNA amplified from a SMART Human Skeletal Muscle cDNA library. Lane 5: 18.5-kb λ insert amplified from a λ clone. Lane M: λ/Hind III DNA size marker.

Back

639207: Advantage 2 PCR Kit

639207: Advantage 2 PCR Kit

Overview

  • Library construction occurs directly in yeast using SMART technology
  • No laborious cloning or library amplification steps
  • Material for hundreds of yeast two-hybrid screens

More Information

Applications

  • Yeast two-hybrid screening

Additional product information

Please see the product's Certificate of Analysis for information about storage conditions, product components, and technical specifications. Please see the Kit Components List to determine kit components. Certificates of Analysis and Kit Components Lists are located under the Documents tab.

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Takara Bio USA, Inc. provides kits, reagents, instruments, and services that help researchers explore questions about gene discovery, regulation, and function. As a member of the Takara Bio Group, Takara Bio USA is part of a company that holds a leadership position in the global market and is committed to improving the human condition through biotechnology. Our mission is to develop high-quality innovative tools and services to accelerate discovery.

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Takara Bio USA, Inc. provides kits, reagents, instruments, and services that help researchers explore questions about gene discovery, regulation, and function. As a member of the Takara Bio Group, Takara Bio USA is part of a company that holds a leadership position in the global market and is committed to improving the human condition through biotechnology. Our mission is to develop high-quality innovative tools and services to accelerate discovery.

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