forward and reverse primer mix Search Results


barcoded forward primer and reverse primer mix biolegio bv  (Biolegio bv)
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Biolegio bv barcoded forward primer and reverse primer mix biolegio bv
Barcoded Forward Primer And Reverse Primer Mix Biolegio Bv, supplied by Biolegio bv, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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quantitect quantiscript reverse-transcriptase and rt primer mix  (Qiagen)
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Qiagen quantitect quantiscript reverse-transcriptase and rt primer mix
Quantitect Quantiscript Reverse Transcriptase And Rt Primer Mix, supplied by Qiagen, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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aurora kinase b forward and reverse primer mix qt00067403  (Qiagen)
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Qiagen aurora kinase b forward and reverse primer mix qt00067403
Aurora Kinase B Forward And Reverse Primer Mix Qt00067403, supplied by Qiagen, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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reverse transcriptase, oligo-dt primers and dntp mix  (Promega)
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Promega reverse transcriptase, oligo-dt primers and dntp mix
Reverse Transcriptase, Oligo Dt Primers And Dntp Mix, supplied by Promega, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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buffered reverse transcriptase quantitect reverse transcriptase, rt buffer, and rt primer mix  (Qiagen)
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Qiagen buffered reverse transcriptase quantitect reverse transcriptase, rt buffer, and rt primer mix
Buffered Reverse Transcriptase Quantitect Reverse Transcriptase, Rt Buffer, And Rt Primer Mix, supplied by Qiagen, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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2× hrm pcr master mix and 10 ρmol of forward and reverse erm(a) and human rnasep primers.  (Qiagen)
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Qiagen 2× hrm pcr master mix and 10 ρmol of forward and reverse erm(a) and human rnasep primers.
2× Hrm Pcr Master Mix And 10 ρmol Of Forward And Reverse Erm(A) And Human Rnasep Primers., supplied by Qiagen, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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oligonucleotide mix  (BioTeZ Inc)
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BioTeZ Inc oligonucleotide mix
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goscripttm reverse transcription mix, random primer protocol, and oligo (dt) protocol  (Promega)
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Promega goscripttm reverse transcription mix, random primer protocol, and oligo (dt) protocol
Goscripttm Reverse Transcription Mix, Random Primer Protocol, And Oligo (Dt) Protocol, supplied by Promega, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
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reverse transcription mix of random nonamers and oligo(dt) primers non/dt  (Qiagen)
90
Qiagen reverse transcription mix of random nonamers and oligo(dt) primers non/dt
TLC1 levels are constant throughout the cell cycle, depressed at saturating cell density, and variable depending on tlc1 allele and plasmid type. (A) FACS analysis of wild-type haploid cells following release from a 3-h arrest in 5 μM α-factor. “1C” indicates haploid DNA content. At each time point shown, cells were removed from culture and either fixed for FACS anlaysis of DNA content or flash-frozen for RNA isolation. The RNA samples were reverse-transcribed using random <t>nonamers</t> and oligo(dT). The resulting cDNA was amplified with three PCR primer sets: p38–39 to quantify TLC1 total, p90–91 to quantify TLC1 3′ extension, and p34–35 to quantify U2. The concentration ratio of TLC1/U2 at each time point was then divided by the concentration ratio of the prearrest sample, i.e., (TLC1/U2)x/(TLC1/U2)pre-arrest, where x is each time point. (B) Graphical representation of TLC1total RNA levels (top) and TLC13′ extension RNA levels (bottom) at the time points shown in A. Each point on the graphs is the mean of two RT-PCR reactions, and the error bars show standard deviation. At each density point, RNA was isolated and reverse-transcribed using random nonamers and oligo(dT). The cDNAs were amplified with the following PCR primer sets: p38–39 to quantify TLC1 total, p32–33 to quantify ACT1 exon, and p34–35 to quantify U2. (C) Graphical representation of normalized TLC1total RNA levels (top) and ACT1 mRNA levels (bottom) at the cell density points shown below the graph. (D) Northern blot analysis of TLC1 RNA over a cell density course. RNA was isolated from the same strain as in C but from an independent cell density course. Note that U2 is used for normalization in real-time RT-PCR experiments because the U2 RNA (1.175 kb) is similar in size to TLC1 (1.167 kb), while U1 is used for normalization in Northern blots because its smaller size (0.568 kb) permits adequate separation from TLC1. (E) Relative TLC1 RNA levels in strains with different genetic contexts or different tlc1 alleles. WT N indicates wild-type haploid; (CEN), low-copy CEN plasmid; (2μ), high-copy 2-micron plasmid; (dex), dextrose media; (raf), raffinose media; (gal), galactose media; WT 2N, wild-type diploid; and Het 2N, TLC1/tlc1Δ heterozygous diploid. Total TLC1 was normalized to U2 as described in Materials and Methods, then the TLC1/U2 concentration ratio of each sample was divided by the concentration ratio of the WT N sample, i.e., (TLC1tot/U2)x/(TLC1tot/U2)WT N, where x is each strain. The TLC13′ extension was normalized to TLC1total, and the resulting percentage of total TLC1 that contains the 3′ extension is shown above each bar. Note that the Y axis is split; the bottom bar extends from 0 to 1, while the upper bar extends from 1 to 27.5.
Reverse Transcription Mix Of Random Nonamers And Oligo(Dt) Primers Non/Dt, supplied by Qiagen, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/reverse transcription mix of random nonamers and oligo(dt) primers non/dt/product/Qiagen
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forward and reverse primer mix  (GenScript corporation)
90
GenScript corporation forward and reverse primer mix
TLC1 levels are constant throughout the cell cycle, depressed at saturating cell density, and variable depending on tlc1 allele and plasmid type. (A) FACS analysis of wild-type haploid cells following release from a 3-h arrest in 5 μM α-factor. “1C” indicates haploid DNA content. At each time point shown, cells were removed from culture and either fixed for FACS anlaysis of DNA content or flash-frozen for RNA isolation. The RNA samples were reverse-transcribed using random <t>nonamers</t> and oligo(dT). The resulting cDNA was amplified with three PCR primer sets: p38–39 to quantify TLC1 total, p90–91 to quantify TLC1 3′ extension, and p34–35 to quantify U2. The concentration ratio of TLC1/U2 at each time point was then divided by the concentration ratio of the prearrest sample, i.e., (TLC1/U2)x/(TLC1/U2)pre-arrest, where x is each time point. (B) Graphical representation of TLC1total RNA levels (top) and TLC13′ extension RNA levels (bottom) at the time points shown in A. Each point on the graphs is the mean of two RT-PCR reactions, and the error bars show standard deviation. At each density point, RNA was isolated and reverse-transcribed using random nonamers and oligo(dT). The cDNAs were amplified with the following PCR primer sets: p38–39 to quantify TLC1 total, p32–33 to quantify ACT1 exon, and p34–35 to quantify U2. (C) Graphical representation of normalized TLC1total RNA levels (top) and ACT1 mRNA levels (bottom) at the cell density points shown below the graph. (D) Northern blot analysis of TLC1 RNA over a cell density course. RNA was isolated from the same strain as in C but from an independent cell density course. Note that U2 is used for normalization in real-time RT-PCR experiments because the U2 RNA (1.175 kb) is similar in size to TLC1 (1.167 kb), while U1 is used for normalization in Northern blots because its smaller size (0.568 kb) permits adequate separation from TLC1. (E) Relative TLC1 RNA levels in strains with different genetic contexts or different tlc1 alleles. WT N indicates wild-type haploid; (CEN), low-copy CEN plasmid; (2μ), high-copy 2-micron plasmid; (dex), dextrose media; (raf), raffinose media; (gal), galactose media; WT 2N, wild-type diploid; and Het 2N, TLC1/tlc1Δ heterozygous diploid. Total TLC1 was normalized to U2 as described in Materials and Methods, then the TLC1/U2 concentration ratio of each sample was divided by the concentration ratio of the WT N sample, i.e., (TLC1tot/U2)x/(TLC1tot/U2)WT N, where x is each strain. The TLC13′ extension was normalized to TLC1total, and the resulting percentage of total TLC1 that contains the 3′ extension is shown above each bar. Note that the Y axis is split; the bottom bar extends from 0 to 1, while the upper bar extends from 1 to 27.5.
Forward And Reverse Primer Mix, supplied by GenScript corporation, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/forward and reverse primer mix/product/GenScript corporation
Average 90 stars, based on 1 article reviews
forward and reverse primer mix - by Bioz Stars, 2026-03
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quantiscript reverse transcriptase and reverse transcription (rt) primer mix (quantitect rt kit, qiagen)  (Qiagen)
90
Qiagen quantiscript reverse transcriptase and reverse transcription (rt) primer mix (quantitect rt kit, qiagen)
TLC1 levels are constant throughout the cell cycle, depressed at saturating cell density, and variable depending on tlc1 allele and plasmid type. (A) FACS analysis of wild-type haploid cells following release from a 3-h arrest in 5 μM α-factor. “1C” indicates haploid DNA content. At each time point shown, cells were removed from culture and either fixed for FACS anlaysis of DNA content or flash-frozen for RNA isolation. The RNA samples were reverse-transcribed using random <t>nonamers</t> and oligo(dT). The resulting cDNA was amplified with three PCR primer sets: p38–39 to quantify TLC1 total, p90–91 to quantify TLC1 3′ extension, and p34–35 to quantify U2. The concentration ratio of TLC1/U2 at each time point was then divided by the concentration ratio of the prearrest sample, i.e., (TLC1/U2)x/(TLC1/U2)pre-arrest, where x is each time point. (B) Graphical representation of TLC1total RNA levels (top) and TLC13′ extension RNA levels (bottom) at the time points shown in A. Each point on the graphs is the mean of two RT-PCR reactions, and the error bars show standard deviation. At each density point, RNA was isolated and reverse-transcribed using random nonamers and oligo(dT). The cDNAs were amplified with the following PCR primer sets: p38–39 to quantify TLC1 total, p32–33 to quantify ACT1 exon, and p34–35 to quantify U2. (C) Graphical representation of normalized TLC1total RNA levels (top) and ACT1 mRNA levels (bottom) at the cell density points shown below the graph. (D) Northern blot analysis of TLC1 RNA over a cell density course. RNA was isolated from the same strain as in C but from an independent cell density course. Note that U2 is used for normalization in real-time RT-PCR experiments because the U2 RNA (1.175 kb) is similar in size to TLC1 (1.167 kb), while U1 is used for normalization in Northern blots because its smaller size (0.568 kb) permits adequate separation from TLC1. (E) Relative TLC1 RNA levels in strains with different genetic contexts or different tlc1 alleles. WT N indicates wild-type haploid; (CEN), low-copy CEN plasmid; (2μ), high-copy 2-micron plasmid; (dex), dextrose media; (raf), raffinose media; (gal), galactose media; WT 2N, wild-type diploid; and Het 2N, TLC1/tlc1Δ heterozygous diploid. Total TLC1 was normalized to U2 as described in Materials and Methods, then the TLC1/U2 concentration ratio of each sample was divided by the concentration ratio of the WT N sample, i.e., (TLC1tot/U2)x/(TLC1tot/U2)WT N, where x is each strain. The TLC13′ extension was normalized to TLC1total, and the resulting percentage of total TLC1 that contains the 3′ extension is shown above each bar. Note that the Y axis is split; the bottom bar extends from 0 to 1, while the upper bar extends from 1 to 27.5.
Quantiscript Reverse Transcriptase And Reverse Transcription (Rt) Primer Mix (Quantitect Rt Kit, Qiagen), supplied by Qiagen, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/quantiscript reverse transcriptase and reverse transcription (rt) primer mix (quantitect rt kit, qiagen)/product/Qiagen
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kasp primer mix (containing 12 μm of each allele-specific forward primer and 30 μm reverse primer diluted in 10 mm tris, ph 8.3)  (LGC Limited)
90
LGC Limited kasp primer mix (containing 12 μm of each allele-specific forward primer and 30 μm reverse primer diluted in 10 mm tris, ph 8.3)
TLC1 levels are constant throughout the cell cycle, depressed at saturating cell density, and variable depending on tlc1 allele and plasmid type. (A) FACS analysis of wild-type haploid cells following release from a 3-h arrest in 5 μM α-factor. “1C” indicates haploid DNA content. At each time point shown, cells were removed from culture and either fixed for FACS anlaysis of DNA content or flash-frozen for RNA isolation. The RNA samples were reverse-transcribed using random <t>nonamers</t> and oligo(dT). The resulting cDNA was amplified with three PCR primer sets: p38–39 to quantify TLC1 total, p90–91 to quantify TLC1 3′ extension, and p34–35 to quantify U2. The concentration ratio of TLC1/U2 at each time point was then divided by the concentration ratio of the prearrest sample, i.e., (TLC1/U2)x/(TLC1/U2)pre-arrest, where x is each time point. (B) Graphical representation of TLC1total RNA levels (top) and TLC13′ extension RNA levels (bottom) at the time points shown in A. Each point on the graphs is the mean of two RT-PCR reactions, and the error bars show standard deviation. At each density point, RNA was isolated and reverse-transcribed using random nonamers and oligo(dT). The cDNAs were amplified with the following PCR primer sets: p38–39 to quantify TLC1 total, p32–33 to quantify ACT1 exon, and p34–35 to quantify U2. (C) Graphical representation of normalized TLC1total RNA levels (top) and ACT1 mRNA levels (bottom) at the cell density points shown below the graph. (D) Northern blot analysis of TLC1 RNA over a cell density course. RNA was isolated from the same strain as in C but from an independent cell density course. Note that U2 is used for normalization in real-time RT-PCR experiments because the U2 RNA (1.175 kb) is similar in size to TLC1 (1.167 kb), while U1 is used for normalization in Northern blots because its smaller size (0.568 kb) permits adequate separation from TLC1. (E) Relative TLC1 RNA levels in strains with different genetic contexts or different tlc1 alleles. WT N indicates wild-type haploid; (CEN), low-copy CEN plasmid; (2μ), high-copy 2-micron plasmid; (dex), dextrose media; (raf), raffinose media; (gal), galactose media; WT 2N, wild-type diploid; and Het 2N, TLC1/tlc1Δ heterozygous diploid. Total TLC1 was normalized to U2 as described in Materials and Methods, then the TLC1/U2 concentration ratio of each sample was divided by the concentration ratio of the WT N sample, i.e., (TLC1tot/U2)x/(TLC1tot/U2)WT N, where x is each strain. The TLC13′ extension was normalized to TLC1total, and the resulting percentage of total TLC1 that contains the 3′ extension is shown above each bar. Note that the Y axis is split; the bottom bar extends from 0 to 1, while the upper bar extends from 1 to 27.5.
Kasp Primer Mix (Containing 12 μm Of Each Allele Specific Forward Primer And 30 μm Reverse Primer Diluted In 10 Mm Tris, Ph 8.3), supplied by LGC Limited, used in various techniques. Bioz Stars score: 90/100, based on 1 PubMed citations. ZERO BIAS - scores, article reviews, protocol conditions and more
https://www.bioz.com/result/kasp primer mix (containing 12 μm of each allele-specific forward primer and 30 μm reverse primer diluted in 10 mm tris, ph 8.3)/product/LGC Limited
Average 90 stars, based on 1 article reviews
kasp primer mix (containing 12 μm of each allele-specific forward primer and 30 μm reverse primer diluted in 10 mm tris, ph 8.3) - by Bioz Stars, 2026-03
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Image Search Results


TLC1 levels are constant throughout the cell cycle, depressed at saturating cell density, and variable depending on tlc1 allele and plasmid type. (A) FACS analysis of wild-type haploid cells following release from a 3-h arrest in 5 μM α-factor. “1C” indicates haploid DNA content. At each time point shown, cells were removed from culture and either fixed for FACS anlaysis of DNA content or flash-frozen for RNA isolation. The RNA samples were reverse-transcribed using random nonamers and oligo(dT). The resulting cDNA was amplified with three PCR primer sets: p38–39 to quantify TLC1 total, p90–91 to quantify TLC1 3′ extension, and p34–35 to quantify U2. The concentration ratio of TLC1/U2 at each time point was then divided by the concentration ratio of the prearrest sample, i.e., (TLC1/U2)x/(TLC1/U2)pre-arrest, where x is each time point. (B) Graphical representation of TLC1total RNA levels (top) and TLC13′ extension RNA levels (bottom) at the time points shown in A. Each point on the graphs is the mean of two RT-PCR reactions, and the error bars show standard deviation. At each density point, RNA was isolated and reverse-transcribed using random nonamers and oligo(dT). The cDNAs were amplified with the following PCR primer sets: p38–39 to quantify TLC1 total, p32–33 to quantify ACT1 exon, and p34–35 to quantify U2. (C) Graphical representation of normalized TLC1total RNA levels (top) and ACT1 mRNA levels (bottom) at the cell density points shown below the graph. (D) Northern blot analysis of TLC1 RNA over a cell density course. RNA was isolated from the same strain as in C but from an independent cell density course. Note that U2 is used for normalization in real-time RT-PCR experiments because the U2 RNA (1.175 kb) is similar in size to TLC1 (1.167 kb), while U1 is used for normalization in Northern blots because its smaller size (0.568 kb) permits adequate separation from TLC1. (E) Relative TLC1 RNA levels in strains with different genetic contexts or different tlc1 alleles. WT N indicates wild-type haploid; (CEN), low-copy CEN plasmid; (2μ), high-copy 2-micron plasmid; (dex), dextrose media; (raf), raffinose media; (gal), galactose media; WT 2N, wild-type diploid; and Het 2N, TLC1/tlc1Δ heterozygous diploid. Total TLC1 was normalized to U2 as described in Materials and Methods, then the TLC1/U2 concentration ratio of each sample was divided by the concentration ratio of the WT N sample, i.e., (TLC1tot/U2)x/(TLC1tot/U2)WT N, where x is each strain. The TLC13′ extension was normalized to TLC1total, and the resulting percentage of total TLC1 that contains the 3′ extension is shown above each bar. Note that the Y axis is split; the bottom bar extends from 0 to 1, while the upper bar extends from 1 to 27.5.

Journal:

Article Title: Low abundance of telomerase in yeast: Implications for telomerase haploinsufficiency

doi: 10.1261/rna.134706

Figure Lengend Snippet: TLC1 levels are constant throughout the cell cycle, depressed at saturating cell density, and variable depending on tlc1 allele and plasmid type. (A) FACS analysis of wild-type haploid cells following release from a 3-h arrest in 5 μM α-factor. “1C” indicates haploid DNA content. At each time point shown, cells were removed from culture and either fixed for FACS anlaysis of DNA content or flash-frozen for RNA isolation. The RNA samples were reverse-transcribed using random nonamers and oligo(dT). The resulting cDNA was amplified with three PCR primer sets: p38–39 to quantify TLC1 total, p90–91 to quantify TLC1 3′ extension, and p34–35 to quantify U2. The concentration ratio of TLC1/U2 at each time point was then divided by the concentration ratio of the prearrest sample, i.e., (TLC1/U2)x/(TLC1/U2)pre-arrest, where x is each time point. (B) Graphical representation of TLC1total RNA levels (top) and TLC13′ extension RNA levels (bottom) at the time points shown in A. Each point on the graphs is the mean of two RT-PCR reactions, and the error bars show standard deviation. At each density point, RNA was isolated and reverse-transcribed using random nonamers and oligo(dT). The cDNAs were amplified with the following PCR primer sets: p38–39 to quantify TLC1 total, p32–33 to quantify ACT1 exon, and p34–35 to quantify U2. (C) Graphical representation of normalized TLC1total RNA levels (top) and ACT1 mRNA levels (bottom) at the cell density points shown below the graph. (D) Northern blot analysis of TLC1 RNA over a cell density course. RNA was isolated from the same strain as in C but from an independent cell density course. Note that U2 is used for normalization in real-time RT-PCR experiments because the U2 RNA (1.175 kb) is similar in size to TLC1 (1.167 kb), while U1 is used for normalization in Northern blots because its smaller size (0.568 kb) permits adequate separation from TLC1. (E) Relative TLC1 RNA levels in strains with different genetic contexts or different tlc1 alleles. WT N indicates wild-type haploid; (CEN), low-copy CEN plasmid; (2μ), high-copy 2-micron plasmid; (dex), dextrose media; (raf), raffinose media; (gal), galactose media; WT 2N, wild-type diploid; and Het 2N, TLC1/tlc1Δ heterozygous diploid. Total TLC1 was normalized to U2 as described in Materials and Methods, then the TLC1/U2 concentration ratio of each sample was divided by the concentration ratio of the WT N sample, i.e., (TLC1tot/U2)x/(TLC1tot/U2)WT N, where x is each strain. The TLC13′ extension was normalized to TLC1total, and the resulting percentage of total TLC1 that contains the 3′ extension is shown above each bar. Note that the Y axis is split; the bottom bar extends from 0 to 1, while the upper bar extends from 1 to 27.5.

Article Snippet: To determine the concentration ratio of TLC1 to U2 in a total RNA sample, we used a reverse transcription mix of random nonamers and oligo(dT) primers (non/dT, Qiagen) to generate an inclusive cDNA pool.

Techniques: Plasmid Preparation, Isolation, Reverse Transcription, Amplification, Concentration Assay, Reverse Transcription Polymerase Chain Reaction, Standard Deviation, Northern Blot, Quantitative RT-PCR