Mung bean nuclease

Mung bean nuclease (Nuclease MB) is a nuclease derived from sprouts of the mung bean (Vigna radiata) that removes nucleotides in a step-wise manner from single-stranded DNA molecules (ssDNA) and is used in biotechnological applications to remove such ssDNA from a mixture also containing double-stranded DNA (dsDNA). This enzyme is useful for transcript mapping, removal of single-stranded regions in DNA hybrids or single-stranded overhangs produced by restriction enzymes, etc. It has an activity similar to Nuclease S1 (both are EC 3.1.30.1), but it has higher specificity for single-stranded molecules.^[1]

The enzyme degrades single-stranded DNA or RNA to nucleoside 5’-monophosphates, but does not digest double-stranded DNA, double-stranded RNA, or DNA / RNA hybrids. Mung Bean Nuclease catalyzes the specific degradation of single-stranded DNA or RNA, and produces mono and oligonucleotides carrying a 5′-P terminus. Mung bean nuclease has a stringent single-stranded specificity for DNA or RNA.

Mung bean nuclease has an estimated molecular weight of 39 kDa by SDS-PAGE. A glycoprotein, 29% of this mass is sugars.^[2] As of April 2019^[update], the specific gene encoding for this protein is unknown, and all production relies on a purification process on bean sprouts from 1980.^[1] Some is known about its structure, with one exposed Cysteine residue and 3 pairs of disulfide bonds. Some is known about its amino acid composition.^[2]

^ ^a ^b "BRENDA: 3.1.30.1".
^ ^a ^b Eun, HM (1996). "Nucleases". Enzymology primer for recombinant DNA technology. Academic Press. pp. 145–232. doi:10.1016/B978-012243740-3/50006-5. ISBN 978-0-12-243740-3.

[brenda-EC-1] "BRENDA: 3.1.30.1".

[eun-2] Eun, HM (1996). "Nucleases". Enzymology primer for recombinant DNA technology. Academic Press. pp. 145–232. doi:10.1016/B978-012243740-3/50006-5. ISBN 978-0-12-243740-3.

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