|
[article] | Title : |
Optimization of PCR Conditions for DNA Amplification of Common Buckwheat Using EST Primers |
| Material Type: |
printed text |
| Authors: |
Joshi, Bal K., Author ; Kazutoshi, Okuno, Author ; T. Hara, Author |
| Publication Date: |
2007 |
| Article on page: |
1-6 p. |
| Languages : |
English (eng) |
| Keywords: |
Annealing temperature, buckwheat, EST markers, optimization of PCRconditions |
| Abstract: |
Under optimal conditions the PCR reaction is very efficient; microgram quantities may be
synthesized from a single molecule of substrate DNA. DNA of four lines of common
buckwheat (Kyusu, Canada, Miyazaki and Botansoba) was used to optimize PCR reaction
and cycling program of 26 primers for DNA amplification of common buckwheat.
Annealing temperature (Ta), PCR cycle number and MgCl2 concentration were considered
optimum if the single clear band was observed. Of the 26 primers Ta of only 10 primers
could be optimized. Three primer pairs performed best at Ta of 54oC. The optimum
concentration of MgCl2 was found to be 1.5mM for all primer pairs. Similarly the number of
PCR cycles was found to be 40 for all 10 primer pairs except for primer pair 57. Optimized
PCR conditions were used for subsequent studies such as transferability of EST primers to
other Fagopyrum species and construction of linkage map. |
| Link for e-copy: |
http://elibrary.narc.gov.np/?r=17 |
in Nepal Agriculture Research Journal > Vol. 8 (2007) . - 1-6 p.
[article] Optimization of PCR Conditions for DNA Amplification of Common Buckwheat Using EST Primers [printed text] / Joshi, Bal K., Author ; Kazutoshi, Okuno, Author ; T. Hara, Author . - 2007 . - 1-6 p. Languages : English ( eng) in Nepal Agriculture Research Journal > Vol. 8 (2007) . - 1-6 p. | Keywords: |
Annealing temperature, buckwheat, EST markers, optimization of PCRconditions |
| Abstract: |
Under optimal conditions the PCR reaction is very efficient; microgram quantities may be
synthesized from a single molecule of substrate DNA. DNA of four lines of common
buckwheat (Kyusu, Canada, Miyazaki and Botansoba) was used to optimize PCR reaction
and cycling program of 26 primers for DNA amplification of common buckwheat.
Annealing temperature (Ta), PCR cycle number and MgCl2 concentration were considered
optimum if the single clear band was observed. Of the 26 primers Ta of only 10 primers
could be optimized. Three primer pairs performed best at Ta of 54oC. The optimum
concentration of MgCl2 was found to be 1.5mM for all primer pairs. Similarly the number of
PCR cycles was found to be 40 for all 10 primer pairs except for primer pair 57. Optimized
PCR conditions were used for subsequent studies such as transferability of EST primers to
other Fagopyrum species and construction of linkage map. |
| Link for e-copy: |
http://elibrary.narc.gov.np/?r=17 |
|
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