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Yeast one-hybrid system—Matchmaker Gold

Our Matchmaker Gold Yeast One-Hybrid Library Screening System provides a simple and efficient method for identifying and characterizing novel protein-DNA interactions. All Matchmaker Gold Systems use Aureobasidin A resistance (AbAr) as a stringent, highly selective, and easy-to-use reporter. This novel reporter produces very low screening backgrounds, since the Aureobasidin A antibiotic (AbA) efficiently kills yeast lacking AbAr expression.

Our Matchmaker Gold Yeast One-Hybrid Library Screening System provides a simple and efficient method for identifying and characterizing novel protein-DNA interactions. All Matchmaker Gold Systems use Aureobasidin A resistance (AbAr) as a stringent, highly selective, and easy-to-use reporter. This novel reporter produces very low screening backgrounds, since the Aureobasidin A antibiotic (AbA) efficiently kills yeast lacking AbAr expression.

The Matchmaker Gold Yeast One-Hybrid Library Screening System

In the Matchmaker Gold Yeast One-Hybrid Library Screening System, tandem repeats of your DNA target/bait sequence are cloned into the pAbAi reporter vector. To generate your bait-specific reporter strain, the pAbAi vector is then integrated into the genome of Y1HGold yeast using homologous recombination. This strain provides a host for library screening.

One-Step library construction and screening

A cDNA library of potential DNA-binding proteins, which are ultimately expressed as fusions to the yeast GAL4 transcription activation domain (GAL4 AD prey proteins), is constructed directly in the Y1HGold[Bait-AbAi] reporter strain using SMART technology and homologous recombination. When a prey protein binds to the bait sequence, its associated GAL4 AD activates AbAr expression, allowing the cell to grow on medium containing AbA. In library screens, the plasmids encoding the library-derived prey proteins can be easily rescued from the surviving yeast clones and subjected to further analysis.

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Cat. # Product Size Price License Quantity Details
630491 Matchmaker® Gold Yeast One-Hybrid Library Screening System 5 Rxns USD $2126.00

A simple and highly efficient system for the simultaneous construction and screening of a cDNA library for protein-DNA interactions. SMART cDNA is synthesized from your RNA sample and then used to construct a library directly in a Y1HGold yeast reporter strain containing your DNA sequence of interest. Positive protein-DNA interactions from the library convey resistance to the yeast antibiotic, Aureobasidin A (AbA).

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 You May Also Like Image Data

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Use colony PCR to quickly analyze your bait-specific reporter strains and sort your positive candidate clones

Use colony PCR to quickly analyze your bait-specific reporter strains and sort your positive candidate clones
Use colony PCR to quickly analyze your bait-specific reporter strains and sort your positive candidate clones. Panel A: Colony PCR was performed using Matchmaker Insert Check PCR Mix 1 to analyze the insertion sites of Y1HGold pAbAi integrant strains, which contain the pAbAi reporter vector with or without a bait sequence (i.e., three tandem repeats of either the Oct4 or p53 binding site). Lane 1: Y1HGold. Lane 2: Y1HGold [AbAi]. Lane 3: Y1HGold [3xOct4-AbAi]. Lane 4: Y1HGold [3xp53-AbAi]. Lane M: 1 kb ladder. The strain lacking pAbAi produced no PCR product, while those containing pAbAi integrants generated amplicons of approximately 1.4 kb. Panel B: Matchmaker Insert Check PCR Mix 2 was used to amplify prey vector inserts from 15 randomly selected positive colonies obtained using a Matchmaker Gold Screening System (Lanes 3-17). The results allowed the clones to be quickly sorted for further analysis. Lane 1: No template control. Lanes M and M2: 1 kb ladder. Lane M1: 100 bp ladder.

Back

Use SMART technology and yeast biology to construct and screen your library

Use SMART technology and yeast biology to construct and screen your library
Use SMART technology and yeast biology to construct and screen your library. Your library is simultaneously constructed and screened directly in yeast. First, SMART cDNA synthesis technology is used to create a pool of cDNA that is flanked by sequence that is homologous to that at the ends of the linearized prey vector, pGADT7-Rec. Next, the newly created Y1HGold-Bait reporter strain is cotransformed with the cDNA pool and pGADT7-Rec, which undergo homologous recombination within the yeast. The yeast cells are then plated on SD/-Leu/+AbA to select for colonies that have an active reporter (i.e., positive Y1H interactions)

Back

Screening for protein-DNA interactions with the Matchmaker Gold One-Hybrid System

Screening for protein-DNA interactions with the Matchmaker Gold One-Hybrid System
Screening for protein-DNA interactions with the Matchmaker Gold One-Hybrid System. One to three copies of the DNA target sequence are cloned into the pAbAi reporter vector, which is then integrated into the Y1HGold genome to create a bait-specific reporter strain. Activation of the AbA resistance gene occurs if a prey protein from the library binds to the bait sequence.

Back

630491: Matchmaker Gold Yeast One-Hybrid Library Screening System

630491: Matchmaker Gold Yeast One-Hybrid Library Screening 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

Back

639206: Advantage 2 PCR Kit

639206: Advantage 2 PCR Kit

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.
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
630496 Matchmaker® Insert Check PCR Mix 1 100 Rxns USD $203.00

Matchmaker Insert Check PCR Mix 1 is a 2X pre-mix that allows quick and easy PCR directly from yeast colonies. The Mix contains a PCR polymerase, primers, dNTPs and buffer; simply add cells to the mix and perform 30 cycles of PCR. Matchmaker Insert Check PCR Mix 1 is designed to be used with our Matchmaker Gold Yeast One-Hybrid Library Screening System (Cat. No. 630491) to confirm the integration site of the pAbAi vector containing your DNA sequence of interest.

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

Back

Use colony PCR to quickly analyze your bait-specific reporter strains and sort your positive candidate clones

Use colony PCR to quickly analyze your bait-specific reporter strains and sort your positive candidate clones
Use colony PCR to quickly analyze your bait-specific reporter strains and sort your positive candidate clones. Panel A: Colony PCR was performed using Matchmaker Insert Check PCR Mix 1 to analyze the insertion sites of Y1HGold pAbAi integrant strains, which contain the pAbAi reporter vector with or without a bait sequence (i.e., three tandem repeats of either the Oct4 or p53 binding site). Lane 1: Y1HGold. Lane 2: Y1HGold [AbAi]. Lane 3: Y1HGold [3xOct4-AbAi]. Lane 4: Y1HGold [3xp53-AbAi]. Lane M: 1 kb ladder. The strain lacking pAbAi produced no PCR product, while those containing pAbAi integrants generated amplicons of approximately 1.4 kb. Panel B: Matchmaker Insert Check PCR Mix 2 was used to amplify prey vector inserts from 15 randomly selected positive colonies obtained using a Matchmaker Gold Screening System (Lanes 3-17). The results allowed the clones to be quickly sorted for further analysis. Lane 1: No template control. Lanes M and M2: 1 kb ladder. Lane M1: 100 bp ladder.

Back

Use SMART technology and yeast biology to construct and screen your library

Use SMART technology and yeast biology to construct and screen your library
Use SMART technology and yeast biology to construct and screen your library. Your library is simultaneously constructed and screened directly in yeast. First, SMART cDNA synthesis technology is used to create a pool of cDNA that is flanked by sequence that is homologous to that at the ends of the linearized prey vector, pGADT7-Rec. Next, the newly created Y1HGold-Bait reporter strain is cotransformed with the cDNA pool and pGADT7-Rec, which undergo homologous recombination within the yeast. The yeast cells are then plated on SD/-Leu/+AbA to select for colonies that have an active reporter (i.e., positive Y1H interactions)

Back

Screening for protein-DNA interactions with the Matchmaker Gold One-Hybrid System

Screening for protein-DNA interactions with the Matchmaker Gold One-Hybrid System
Screening for protein-DNA interactions with the Matchmaker Gold One-Hybrid System. One to three copies of the DNA target sequence are cloned into the pAbAi reporter vector, which is then integrated into the Y1HGold genome to create a bait-specific reporter strain. Activation of the AbA resistance gene occurs if a prey protein from the library binds to the bait sequence.

Back

630496: Matchmaker Insert Check PCR Mix 1

630496: Matchmaker Insert Check PCR Mix 1

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

Back

639206: Advantage 2 PCR Kit

639206: Advantage 2 PCR Kit

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.
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

  • Highest-performing yeast one-hybrid system
  • Aureobasidin A selection eliminates screening background
  • Construct and screen SMART cDNA libraries directly in yeast

More Information

Applications

  • Yeast one-hybrid screening

Get results fast!

With the Matchmaker Gold system, one-hybrid library screening is straightforward, quick, and easy:

Step 1: Create a bait construct by cloning 1–3 tandem repeats of the target DNA-binding sequence into pAbAi.

Step 2: Create a bait-specific reporter strain by transforming and integrating the linearized pBait-AbAi construct into the Y1H Gold yeast strain and selecting on SD/–Ura agar medium.

Step 3: Confirm the integration of the bait sequence using colony PCR and the Matchmaker Insert Check PCR Mix 1.

Step 4: Use SMART technology to synthesize cDNA containing ends that are homologous to the ends of the linearized pGADT7-Rec vector.

Step 5: Create and screen your library in a single step by cotransforming your bait-specific reporter strain with the SMART-generated cDNA and the linearized pGADT7-Rec vector, and plating on AbA-containing selective medium.

Step 6: Harvest the resulting colonies, which contain putative DNA-binding prey proteins, and analyze your library inserts using the Matchmaker Insert Check PCR Mix 2.

Analysis by colony PCR

Screening positive colonies by PCR is a fast and convenient way to analyze the bait strain and sort through the positive clones identified in Y1H and Y2H screens. With the Matchmaker Insert Check PCR Mix 1, you can verify the integration of your Y1H pBait-AbAi construct, and with the companion Matchmaker Insert Check PCR Mix 2, you can quickly sort through and analyze the inserts in positive clones that have emerged from either one-hybrid or two-hybrid screens.

Yeast one-hybrid media

Our yeast one-hybrid media sets each contain a complete set of all the yeast media pouches you need for Matchmaker Gold One-Hybrid protocols.

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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What does it take to generate good science? Careful planning, dedicated researchers, and the right tools. At Takara Bio, we thoughtfully develop exceptional products to tackle your most challenging research problems, and have an expert team of technical support professionals to help you along the way, all at superior value.

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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.

FOR RESEARCH USE ONLY. NOT FOR USE IN DIAGNOSTIC PROCEDURES (EXCEPT AS SPECIFICALLY NOTED).

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