Modern Applications of DNA Amplification Techniques 1997
DOI: 10.1007/978-1-4615-5379-3_9
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The Effect of Quantitative Ratio Between Primer Pairs on Pcr Products in Multi-Target Amplification

Dani Bercovich
1
,
Zipi Regev
2
,
Tal Ratz
3
et al.
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“…Amplification of the 18S rRNA cDNA in the same tube with either GtH-I or GtH-II cDNA caused a reduction in one or both PCR products. Such interference problems are not uncommon in multiplex PCR, as reported by Bercovich et al (1997). We have carefully calibrated the concentration of each primer pair and the number of cycles for amplifications which were linearly dependent on the initial concentration of the target cDNA.…”
Section: Amplification Of the Cdna Of Gth-i Gth-ii And 18s Rrna Eachmentioning
confidence: 99%

Blue gourami (Trichogaster trichopterus) gonadotropic beta subunits (I and II) cDNA sequences and expression during oogenesis

Jackson
1
,
Goldberg2,
Ofir3
et al. 1999
Journal of Molecular Endocrinology
60
5
53
0
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“…Amplification of the 18S rRNA cDNA in the same tube with either GtH-I or GtH-II cDNA caused a reduction in one or both PCR products. Such interference problems are not uncommon in multiplex PCR, as reported by Bercovich et al (1997). We have carefully calibrated the concentration of each primer pair and the number of cycles for amplifications which were linearly dependent on the initial concentration of the target cDNA.…”
Section: Amplification Of the Cdna Of Gth-i Gth-ii And 18s Rrna Eachmentioning
confidence: 99%

Blue gourami (Trichogaster trichopterus) gonadotropic beta subunits (I and II) cDNA sequences and expression during oogenesis

Jackson
1
,
Goldberg2,
Ofir3
et al. 1999
Journal of Molecular Endocrinology
60
5
53
0
View full textAdd to dashboardCite
show abstract
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