Digestion of DNA with Restriction Endonucleases

@article{Bloch2001DigestionOD,
  title={Digestion of DNA with Restriction Endonucleases},
  author={Kenneth D. Bloch},
  journal={Current Protocols in Immunology},
  year={2001},
  volume={2}
}
  • K. D. Bloch
  • Published 1 June 1992
  • Biology
  • Current Protocols in Immunology
Restriction endonucleases recognize short DNA sequences and catalyze the cleavage of double‐stranded DNA at specific sites within or adjacent to the recognition sequences. This unit describes how to cleave DNA and refers the investigator to frequently updated manuals by endonuclease suppliers for the precise optimized conditions. Alternate procedures are given for digesting a DNA sample with several different enzymes and digesting multiple DNA samples with the same endonuclease. 
View on Wiley
people.rit.edu
19 Citations
Highly Influential Citations
5
Background Citations
6
Methods Citations
8

19 Citations

Citation Type

Citation Type

Sequencing by ligation variation with endonuclease V digestion and deoxyinosine-containing query oligonucleotides
TLDR
This work describes a variation on traditional SBL protocols that extends the number of sequential bases that can be sequenced by using Endonuclease V to nick a query primer, thus leaving a ligatable end extended into the unknown sequence for further SBL cycles.
Principles and Applications of PRINS in Cytogenetics
  • J. Koch
  • Biology
    Current protocols in human genetics
  • 2004
TLDR
This unit describes basic PRINS and the alternative version, dideoxy‐PRINS, which can increase the sensitivity of the reaction by an order of magnitude.
Principles and Applications of PRINS in Cytogenetics
  • J. Koch
  • Biology
    Current protocols in cytometry
  • 2004
TLDR
This unit describes basic PRINS and the alternative version, dideoxy‐PRINS, which can increase the sensitivity of the reaction by an order of magnitude.
Working with Enzymes
TLDR
The basic general principles of enzymes are applied to a specific class of enzymes, called restriction endonucleases, in order to demonstrate how to correctly set up an enzymatic reaction.
Expression and purification of recombinant proteins by fusion to maltose-binding protein
  • P. Riggs
  • Biology
    Molecular biotechnology
  • 2000
TLDR
Vectors with or without the malE signal sequence can be used, to express the protein cytoplasmically for the highest level of production or periplasmically to help in proper folding of disulfide-bonded proteins.
Cloning of bHLH promoter fragment in pGEMT vector using E. coli (Migula) strain for various stress tolerance in chickpea
TLDR
Genomic DNA of chickpea was isolated for bHLH promoter and amplicon of size 1.7 kb was obtained by PCR of template DNA and its ligation with pGEMT vector was performed for cloning to confirm the presence of insert.
Detection of Isotype Switch Rearrangement in Bulk Culture by PCR
TLDR
The protocols in this unit describe two polymerase chain reaction (PCR)‐based strategies for detecting switch rearrangements in bulk culture that are capable of detecting reciprocal deletion circles as well as functional recombination products remaining on the expressed chromosome.
Transfection by Electroporation
TLDR
Electroporation of mammalian cells, including ES cells for the preparation of knock‐out, knock‐in, and transgenic mice, and modifications for preparation and transfection of plant protoplasts are described.
Transfection by Electroporation
TLDR
Electroporation of mammalian cells, including ES cells for the preparation of knock‐out, knock‐in, and transgenic mice, and modifications for preparation and transfection of plant protoplasts are described.
Analysis of Membrane Protein Interactions with a Bacterial Adenylate Cyclase–Based Two‐Hybrid (BACTH) Technique
TLDR
This unit describes the basic procedures to characterize protein‐protein interactions with the BACTH genetic system and to search for potential partners of known proteins.
...
1
2
...

References

SHOWING 1-7 OF 7 REFERENCES
Guide to the use of type II restriction endonucleases.
A nomenclature for restriction enzymes, DNA methyltransferases, homing endonucleases and their genes.
A nomenclature is described for restriction endonucleases, DNA methyltransferases, homing endonucleases and related genes and gene products. It provides explicit categories for the many different
KGB: a single buffer for all restriction endonucleases
TLDR
Testing fifty-five restriction endonucleases for their ability to cleave DNA in a series of KGlu buffers and the level of activity was compared with that found under conditions recommended by the vendors.
Restriction enzymes and their isoschizomers.
TLDR
In forming this list, all endonucleases cleaving DNA at a specific sequence have been considered to be restriction enzymes, although in most cases there is no direct genetic evidence for the presence of a restriction-modification system.
Biotech Buyers' Guide
  • 1991
Advanced bacterial genetics
Molecular cloning.