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Home Q&AWhy do we get eluted plasmid contaminated with RNA?

Plasmid DNA Extraction Kit(PD004, PD100, PD300) --Q&A
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Q Can the plasmid DNA extraction Kit be applied on Gram (+) bacteria?
Q Why do we get eluted plasmid contaminated with RNA?
A Make sure that RNase A is added into PD1 (or PM1) Buffer. Store the PD1 (or PM1) Buffer at 4˚C. If RNase A-added PD1 (PM1) Buffer is not properly stored at 4˚C or has been stored for a long time (e.g., more than 6 months) RNase A activity may have been reduced, thus not being able to degrade RNA completely. In this case, fresh RNase A has to be added into PD1 (PM1) Buffer with a final concentration of 50 mg/ml. Again, store the buffer at 4˚C.
Q Why can¡¦t the eluted plasmid be cut by restriction enzymes properly?
Q Why does the Plasmid DNA Extraction Kit require two washings with two types of wash buffers (W1 and Wash Buffer) while competitors kits require one washing?
Q Eluted plasmid appeared degraded after storage for an extended period of time.
Q Why was Restriction enzyme digestion unsuccessful?

Genomic DNA Extraction Kit(GT004,GT050,GT300,GB004,GB100,GB300,GP004,GP100)--Q&A
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Q Why doesn¡¦t the Eluted DNA perform well in downstream applications?
Q Why does the genomic DNA band appear smeared in agarose gel electrophoresis?
Q What is the key to successfully isolating genomic DNA of good yield and quality?
Q Why does the sample appear viscous after sample Lysis and not pass through the column easily, even when less than the suggested maximum sample amount is used?
Q When Buffy coat is used, the column tends to be clogged.

Gel/PCR DNA Fragments Extraction Kit (DF004, DF100, DF300)--Q&A

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