I have problem for removing polysccharides in the dna extraction of bacteria. when I want to collect supernatant after adding extraction buffer, suppernatant isn't sufficient and DNA concentration is law and isn't sharp. But RNA qualifiction and quantification is better than DNA. Can anyone help me how can I improve the quantication of DNA?
The addition of NaCl at concentrations higher than 0.5 M, along with CTAB, is known to remove polysaccharides during DNA extraction:
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Not sure if you do it manually or with DNA prep kits but CTAB is a good detergent to use around the protease treatment step.
(Wilson K. Preparation of genomic DNA from bacteria. Curr Protoc Mol Biol. 2001 Nov;Chapter 2:Unit 2.4. doi: 10.1002/0471142727.mb0204s56. PMID: 18265184.)
Bacteria are lysed by freezing and grinding in liquid nitrogen, and treated with SDS. A phenol/chloroform mixture is used to purify the extracted DNA, and Isopropanol is used to precipitate the result. Article A simple method for DNA extraction from marine bacteria that...
Polysaccharides can be a common contaminant in bacterial DNA extraction, particularly when working with certain types of bacterial cells or tissues. These polysaccharides can interfere with downstream applications such as PCR or sequencing.
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