Molecular Cloning: A Laboratory Manual, Book 2 |
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Page 50
Today , the secondary ligand is covalently linked to an enzyme whose activity
can be detected histochemically ( e . g . , alkaline ... Because such antisera
normally react with many different epitopes , the chances of detecting a cDNA
clone that ...
Today , the secondary ligand is covalently linked to an enzyme whose activity
can be detected histochemically ( e . g . , alkaline ... Because such antisera
normally react with many different epitopes , the chances of detecting a cDNA
clone that ...
Page 31
The amount of genomic DNA needed to generate a detectable hybridization
signal depends on a number of factors ... A sequence of 1000 bp that occurs only
once in the mammalian genome ( i . e . , 1 part in 3 million ) can be detected in an
...
The amount of genomic DNA needed to generate a detectable hybridization
signal depends on a number of factors ... A sequence of 1000 bp that occurs only
once in the mammalian genome ( i . e . , 1 part in 3 million ) can be detected in an
...
Page 56
Hybridization of Radiolabeled Oligonucleotides to Genomic DNA Oligonucleotide
probes as short as 17 nucleotides in length may be used to detect single - copy
sequences in restriction digests of eukaryotic genomic DNA that have been ...
Hybridization of Radiolabeled Oligonucleotides to Genomic DNA Oligonucleotide
probes as short as 17 nucleotides in length may be used to detect single - copy
sequences in restriction digests of eukaryotic genomic DNA that have been ...
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User Review - iayork - LibraryThingthe BIBLE of every biologist: So few and so much to say about this bible of Biology at the bench... You'll really find everything you want in it, including the composition of all the buffers and ... Read full review
Contents
TEST LIGATION 3 29 | 3 |
SYNTHESIS OF THE FIRST STRAND OF cDNA 8 | 11 |
FRAGMENT OF E coli DNA POLYMERASE I 13 59 | 14 |
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Common terms and phrases
acid activity agarose aliquots allow amount amplification appropriate approximately bacteriophage bacteriophage T4 base buffer carried cDNA cells centrifugation Chapter chromatography cleaved clones colonies concentration constructed containing deletions denatured described determine digestion DNA polymerase dNTPs double-stranded efficiency electrophoresis et al ethanol expression Figure filters fragment gene genomic hybridization increase Incubate inserted interest isolated labeled length libraries ligation linear linkers method microfuge minutes mixture molecules mRNA mutagenesis mutagenic mutations Nucleic nucleotides obtained oligonucleotide original plaques plasmid plasmid DNA plate pool position possible prepared presence primer probe problem protein purified radiolabeled reaction recombinant region remove restriction enzyme room temperature samples screening sequence single single-stranded solution specific step Store strand synthesis target DNA target sequence template termini tion transfer transformants tube units usually vector volume
References to this book
Bibliographic information
| Title | Molecular Cloning: A Laboratory Manual, Book 2 Molecular Cloning: A Laboratory Manual, Joseph Sambrook, ISBN 0879693096, 9780879693091 |
| Authors | Joseph Sambrook, E. F. Fritsch, Tom Maniatis |
| Edition | 2 |
| Publisher | Cold Spring Harbor Laboratory, 1989 |
| Original from | the University of Michigan |
| Digitized | 15 Jul 2008 |
| ISBN | 0879693096, 9780879693091 |
| Length | 654 pages |
| Export Citation | BiBTeX EndNote RefMan |