New Products

High-capacity version of DNA Cleanup for purification and concentration of DNA up to 100 μg from various sample types, featuring precision-engineered spin columns.

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The NEBNext^® Enzymatic Methyl-seq v2 Conversion Module contains reagents for enzyme-based conversion for methylome analysis, with an expanded input range.

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New version of Monarch kit for total RNA purification and extraction from a variety of sample types including cells, blood, tissue, plants, bacteria, and more using spin column method.

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High-fidelity isoschizomer of LguI and SapI, used in linearization of plasmid DNA for mRNA therapeutics; recognizes the sequence GCTCTTCN^NNN_.

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Monarch Buffer BY included in Monarch kits, available for purchase separately.

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RNase 4 Digestion and 3´ End Repair Mix is a coformulation of RNase 4 and T4 Polynucleotide Kinase that simplifies RNase 4 digestion products into a pool of U-ending RNA oligonucleotides with homogeneous 3´-hydroxy termini.

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The NEBNext^® Enzymatic Methyl-seq v2 Kit contains reagents for enzyme-based specific detection of 5mC and 5hmC, with an expanded input range and more streamlined workflow.

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Endoglycosidase that hydrolyzes internal β(1-4)-galactose linkages within a variety of sulfated and nonsulfated poly-N-acetyllactosamine structures.

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Modified NTPs are commonly used for reduction of immunogenicity for in vitro transcription RNA.

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Modified NTPs are commonly used for reduction of immunogenicity for in vitro transcription RNA.

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Modified NTPs are commonly used for reduction of immunogenicity for in vitro transcription RNA.

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RT-PCR primer set for use upstream of RSV library prep and sequencing on Illumina or Oxford Nanopore Technologies platforms

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GMP-grade Salt Active Nuclease for AAV, protein & biopharma manufacturing at high salt for nucleic acid removal. Up to 2X higher activity than other nucleases.

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Proprietary endonuclease that non-specifically cleaves and degrades all forms of DNA and RNA, with optimal activity in high salt (500 mM NaCl/KCl).

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Thermostable Endonuclease Q is an archaeal DNA endonuclease that cleaves the phosphate backbone of a DNA substrate 5′ to the position of the modified nucleobases of deoxyxanthosine (dX), deoxyinosine (dI), deoxyuracil (dU), and an abasic (AP) site. The result is a 3′-OH and a 5′-phosphate.

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Monarch Buffer BZ included in Monarch kits, also available for purchase separately.

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Monarch Buffer B1 included in Monarch kits available for purchase separately.

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Monarch Buffer B2 included in Monarch kits available for purchase separately.

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Monarch Buffer B3 included in Monarch kits available for purchase separately.

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An engineered variant of Bst DNA Polymerase, Large Fragment optimized for LAMP performance with high specificity and fast polymerization.

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This new module includes the reagents recommended in the updated Oxford Nanopore Technologies^® SQK-LSK114 singleplex ligation sequencing library prep protocols.

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An engineered variant of Bst DNA Polymerase, Large Fragment optimized for LAMP with high specificity and fast polymerization in a glycerol-free format.

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Monarch Spin Columns S3A and Collection Tubes for high-capacity DNA cleanup, available for purchase separately.

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Monarch Buffer WZ included in Monarch kits, available for purchase separately.

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RNase R is a highly processive 3´ to 5´ exoribonuclease that digests linear RNA with an accessible 3´ end and can be used to enrich for circular and lariat RNA.

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The NEBNext Library Quant Kit for Ultima Genomics is a qPCR-based solution for precise and reliable quantitation of NGS libraries prepared using the UG 100 Solaris^TM Free workflow.

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mRNA has emerged as a potent modality for therapeutics. Incorporation of chemically modified ribonucleotides improves the efficacy of these therapies by increasing stability, reducing immunogenicity, and enhancing translatability of mRNAs.

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Cold-active version of TEV protease, designed for higher activity and faster performance at colder temperatures.

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