than 1pmol of template DNA for each sequence (0.25pmol per reaction). See figure 1.
3.
denaturation temperature.
Film blank or very faint1.If using
2.DNA preparation may be bad. Try the control DNA supplied in the kit.
3.Labeled dideoxynucleotide too old. Try longer exposure.
4.Some component missing.
5.Enzyme lost activity.
6.Insufficient template DNA or insufficient number of cycles. Try more DNA, more cycles or longer film exposure.
7.Incorrect temperatures for primers used. Try a lower temperature for cycling (e.g.
8.Incorrect termination time or temperature for dITP. Termination should be 5-
10 minutes at
8.Too little primer used. The recommended amount of primer is
9.Primer bad. Some primers form dimers, hairpins etc., interfering with annealing with the template. Try a different primer.
10.Wrong amounts of dNTP or
1.Too much dNTP or too little
1.Contaminated DNA preparation. Try control DNA. Thermo Sequenase DNA polymerase is sensitive to salt concentration, especially above 75mM.
2.Gel may be bad. Gels should be cast with fresh acrylamide solutions and should polymerize rapidly, within 15 minutes of pouring. Try running a second gel with the same samples.
3.Gel run too cold. Sequencing gels should be run at
4.Gel dried too hot or not flat enough to be evenly exposed to film.
5.Samples not denatured. Make sure samples are always heated to 70°C for at least 2 minutes (longer in an
loading on gel. When
1.Gel compression artifacts. Sometimes a band in all 4 lanes indicates a severe gel compression caused by secondary structures not completely denatured during electrophoresis. If the gel has a region where the bands are very closely spaced, followed by a region where the bands are widely
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