CiNii Books - Gene cloning and manipulation

Author(s)

- Howe, Christopher

Bibliographic Information

Gene cloning and manipulation

Christopher Howe

Cambridge University Press, c1995

hbk
pbk.

Available at / 10 libraries

神戸医療未来大学図書・情報センター

pbk.467.2||H96100071757

OPAC
Kobe University Library for Science and Technology

hbk467-0-48h039600000530*

OPAC
University of Shizuoka Kusanagi Library

hbk467.2||H9696011515

OPAC
城西大学水田記念図書館

hbk0096017660

OPAC
東京大学理学図書館図書

pbk.53:H00:192050000435

OPAC
Toyo University Asaka Library

hbk467.2:HC0400056289

OPAC
日本赤十字広島看護大学図書館

hbk467.21/H96/0009973

OPAC
広島国際大学図書館図

pbk.579.93||H39827867

OPAC
福山大学附属図書館

hbk129701580

OPAC
Meiji University Library生

467.2||58||||S2200001780

OPAC
No Libraries matched.
Remove all filters.

Search this Book/Journal

Note

Includes bibliographical references (p. 195-200) and index

Description and Table of Contents

Description

This text gives a broad, but concise, coverage of gene cloning and manipulation, suitable for undergraduates and beginning graduate students. Assuming only general biochemical knowledge, it stresses the concepts underlying particular types of cloning vector, and uses examples to illustrate them, rather than simply presenting a mass of detailed lists and vector maps. The book starts by describing the principles behind cloning DNA in E. coli, the enzymes used, the range of cloning vectors available, and how to screen libraries to find particular clones. The author shows how PCR can be used as an alternative, or complementary, approach. He then goes on to describe how sequences can be exploited, after cloning and identification, by site-directed mutagenesis and over-expression. The book finishes with a detailed presentation of the genetic manipulation of other organisms, including other bacteria, yeast, plants, insects, and mammals.

Table of Contents

Part I. The Tools for the Job: 1. Introduction
2. Cutting
3. Modification
4. Ligation
5. Purification of plasmid DNA from E. Coli
6. Gel electrophoresis of nucleic acids
7. Oligonucleotide synthesis
Part II. Simple Cloning: 8. The basic experiment
9. Vectors
transformation and hosts
10. Modifications
11. Linkers, adaptors and cassettes
Part III. Other vector systems for E. Coli
12. Introduction
13. Bacteriophage M13 and its uses
14. Bacteriophage lambda
15. Cosmids
16. Bacteriophage P1
Part IV. Making Libraries: 17. Introduction
18. Genomic libraries
19. cDNA libraries
20. Specialized libraries
Part V. Screening Libraries: 21. Introduction
22. Screening for coding function
23. Screening for other functions-reporter genes
Part VI. Polymerase Chain Reaction: 24. The basic technique
25. Modifications
26. Precautions and drawbacks
27. Modification and mutagenesis
28. Introduction
29. Alteration of restriction sites
30. Insertions and deletions
31. Point mutations - early methods
32. Oligonucleotide mutagenesis
33. Choosing the right mutations
34. Inactivating genes
Part VII. Use of Cloned DNA: 35. As DNA
36. Synthesis of RNA
37. Synthesis of protein
Part VIII. Using Other Organisms: 38. Gram-negative bacteria
39. Gram-positive bacteria
40. Fungi
41. Chlamydomonas
42. Vascular plants
43. Organelle transformation
44. Insects
45. Mammals
References and further reading
Index.

by "Nielsen BookData"