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Titlebook: Enzymes of Molecular Biology; Michael M. Burrell Book 1993 Humana Press 1993

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Deoxyribonuclease I (EC 3.1.21.1) and II (EC 3.1.22.1),lar biology, The Type II restriction endonucleases obviously fall into this category, however they are a large subject on their own and therefore are dealt with in a separate section of this book. DNases acting preferentially on single-stranded DNA (ss DNA) substrates are also dealt with in another section of this chapter.
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Outlook: Agile as the New Normal?,homononucleotides. This chapter focuses on the endoribonuclease RNase A (otherwise described as RNase, RNase I, or pancreatic ribonuclease), which shows some base specificity in where it cleaves RNA. The enzyme has been particularly well characterized at the molecular level.
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Agile in der Unternehmenspraxisused, for example, to reveal the protein components of cell organelles by the hydrolysis of tissue slices (.), and as an alternative to proteinase K to remove protein during plasmid DNA (.), chromosomal DNA (.), and RNA isolation (.–.). Another use of pronase is the production of a protein hydrolysate suitable for amino acid analysis (.,.).
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Agile eHealth Usability Evaluationely degrade double-stranded DNA (.–.). Mung-bean nuclease 1 is also reported to show a separate 3′-ω-monophosphatase activity (.) (..). Mung-bean nuclease 1 is a zinc metalloenzyme that requires Zn. and a reducing agent, such as cysteine, for both activity and stability.
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Mung-Bean Nuclease 1 (EC 3.1.30.1),ely degrade double-stranded DNA (.–.). Mung-bean nuclease 1 is also reported to show a separate 3′-ω-monophosphatase activity (.) (..). Mung-bean nuclease 1 is a zinc metalloenzyme that requires Zn. and a reducing agent, such as cysteine, for both activity and stability.
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