Experiment 1: An RT-PCR was run on human cells growing in tissue culture under standard conditions, using the primers described above. A normal PCR was also run on the cells, using the same primers. They were run on an agarose gel shown on the left in the figure (gel 1), in the wells indicated by ‘RT-PCR’ and ‘PCR’. The arrow shows the direction of current in the gel. a) Observe the gel and describe the results for the RT-PCR and PCR (no explanation, just describe). b) Explain why the bands have travelled different distances on the gel.

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Experiment 1:

An RT-PCR was run on human cells growing in tissue culture under standard conditions, using the primers described above. A normal PCR was also run on the cells, using the same primers. They were run on an agarose gel shown on the left in the figure (gel 1), in the wells indicated by ‘RT-PCR’ and ‘PCR’. The arrow shows the direction of current in the gel.

a) Observe the gel and describe the results for the RT-PCR and PCR (no explanation, just

describe).

b) Explain why the bands have travelled different distances on the gel.

Two PCR primers have been designed to the human gene Des23. One primer is reverse complement to a
region including the start codon sequence, and one primer is reverse complement to a region including
the stop codon sequence (and each primer is 20 bp long). These primers have been used in both
experiment one and two.
ATG
STOP
intron 1
exon 2
intron 2
exon 3
intron 3
exon 4
Gel 2
1 2 3 4
exon 1
Gel 1
RT-PCR PCR
Transcribed Image Text:Two PCR primers have been designed to the human gene Des23. One primer is reverse complement to a region including the start codon sequence, and one primer is reverse complement to a region including the stop codon sequence (and each primer is 20 bp long). These primers have been used in both experiment one and two. ATG STOP intron 1 exon 2 intron 2 exon 3 intron 3 exon 4 Gel 2 1 2 3 4 exon 1 Gel 1 RT-PCR PCR
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