Cloning Reagents
Cloning Reagents:
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Restriction Enzymes:
- Enzymes used to cut DNA at specific recognition sequences, facilitating the creation of cohesive ends for ligation.
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DNA Ligase:
- Enzyme responsible for joining DNA fragments by catalyzing the formation of phosphodiester bonds between adjacent nucleotides.
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Polymerases:
- DNA polymerases, such as Taq polymerase or high-fidelity polymerases, are used for amplifying DNA fragments through PCR.
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Nucleotides:
- dNTPs (deoxynucleotide triphosphates) are the building blocks for DNA synthesis in PCR and other enzymatic reactions.
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Competent Cells:
- Host cells that can take up exogenous DNA, commonly used for transformation in cloning experiments.
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Plasmid Extraction Kits:
- Kits containing reagents for isolating plasmid DNA from bacterial cultures, essential for downstream cloning steps.
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PCR Cleanup Kits:
- Kits for purifying PCR products, removing primers, nucleotides, and enzymes to obtain clean DNA fragments for cloning.
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Gel Extraction Kits:
- Kits for purifying DNA fragments from agarose gels, often used after gel electrophoresis to recover specific DNA bands.
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Ligation Buffers and Mixes:
- Buffer solutions optimized for DNA ligation reactions, containing salts and cofactors necessary for efficient ligation.
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Transformation Reagents:
- Chemicals or electroporation solutions used to introduce foreign DNA into host cells during transformation.
Cloning Plasmids:
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pUC Vectors:
- Common cloning vectors with a high copy number and small size, useful for cloning small DNA fragments.
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pBluescript Vectors:
- Cloning vectors based on the pUC backbone, featuring unique restriction sites and a lacZ α-complementation system for blue-white screening.
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pET Vectors:
- Expression vectors designed for protein production in E. coli, featuring strong promoters (e.g., T7 promoter) and fusion tags (e.g., His tag).
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pGEM Vectors:
- Cloning vectors with a high copy number and ampicillin resistance, suitable for routine cloning and sequencing applications.
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Gateway Vectors:
- Vectors designed for Gateway cloning technology, enabling efficient and precise transfer of DNA fragments between different vectors.
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Bacterial Artificial Chromosomes (BACs):
- Large cloning vectors capable of accommodating large DNA inserts (up to hundreds of kilobases) for genomic library construction and functional genomics studies.
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