TY - JOUR
T1 - A simple methodology for RNA isolation from bacteria by integration of formamide extraction and chitosan-modified silica purification
AU - Zhao, Xiaoli
AU - Li, Yong
AU - Duan, Yake
AU - Amin, Amr
AU - Xie, Yingqiu
AU - Shi, Chao
AU - Ma, Cuiping
N1 - Publisher Copyright:
© 2021, Springer-Verlag GmbH Germany, part of Springer Nature.
PY - 2021/11
Y1 - 2021/11
N2 - RNA isolation from bacteria is technically difficult due to the RNA characteristic of labile and vulnerable degradation. Many reagents were explored for cellular lysis and complete inhibition of RNase. However, the available methods for RNA isolation are either of low efficiency or time-consuming. Here, we developed a rapid and accessible protocol for RNA isolation that combined a simplified cell lysis and RNA release by formamide-based solution and RNA purification by chitosan-modified silica membrane for the first time. With this method, we obtained about ~ 28 μg of total RNA from 108Escherichia coli cells. The entire procedure can be done within 15 min without redundant pipetting steps. The purity of extracted RNA was comparable to that of commercial kits, but the cost was much lower. Furthermore, the yielded RNA was successfully used in downstream enzymatic reactions, such as reverse transcription and quantitative real-time PCR. This new method would be of benefit for an extensive range of gene expression analyses in bacterial organisms. Graphical abstract: [Figure not available: see fulltext.]
AB - RNA isolation from bacteria is technically difficult due to the RNA characteristic of labile and vulnerable degradation. Many reagents were explored for cellular lysis and complete inhibition of RNase. However, the available methods for RNA isolation are either of low efficiency or time-consuming. Here, we developed a rapid and accessible protocol for RNA isolation that combined a simplified cell lysis and RNA release by formamide-based solution and RNA purification by chitosan-modified silica membrane for the first time. With this method, we obtained about ~ 28 μg of total RNA from 108Escherichia coli cells. The entire procedure can be done within 15 min without redundant pipetting steps. The purity of extracted RNA was comparable to that of commercial kits, but the cost was much lower. Furthermore, the yielded RNA was successfully used in downstream enzymatic reactions, such as reverse transcription and quantitative real-time PCR. This new method would be of benefit for an extensive range of gene expression analyses in bacterial organisms. Graphical abstract: [Figure not available: see fulltext.]
KW - Bacteria
KW - Chitosan-modified silica membrane
KW - Formamide
KW - Nucleic acid extraction
KW - RNA purification
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U2 - 10.1007/s00216-021-03644-6
DO - 10.1007/s00216-021-03644-6
M3 - Article
C2 - 34505946
AN - SCOPUS:85114697096
SN - 1618-2642
VL - 413
SP - 6469
EP - 6477
JO - Analytical and Bioanalytical Chemistry
JF - Analytical and Bioanalytical Chemistry
IS - 26
ER -