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Extraction RNA Protocol from Blood and Testis Tissue of Local Roosters

Document Type : Articles

Authors

1 Department of Animal Production, College of Agriculture, Tikrit University, Tikrit, Iraq.College of Wildlife Resources Northeast Forestry University Harbin China.

2 Department of Animal Production, College of Agriculture, Tikrit University, Tikrit, Iraq

3 Ministry of Agriculture, Agricultural Research Department, Baghdad, Iraq

Abstract

The (one-step) method has become widely used to isolate total RNA from living organism samples and from different tissues. The aim of this study is to extract RNA from the blood and testicular tissue of male local chickens. The principle behind the method is to separate the RNA from the DNA after extraction with an acid solution containing (Acid guanidinium thiocyanate-phenol-chloroform) with centrifugation, under acidic conditions, the total RNA remains in the upper aqueous phase while most of the acid descends. The DNA and proteins are either in the interphase or in the lower organic phase and then the total RNA is collected by precipitation with isopropanol. Our results showed a significant increase in the concentration of RNA extracted from the blood compared to the testis tissue of local roosters. This protocol made it possible to isolate RNA from cells and tissues in less than 4 hours and was the reason for the great advances in gene expression analysis in plant and animal models, as well as in pathological samples as clearly demonstrated by the huge number of citations the protocol has gained in the past 20 years.

Keywords

References
  1. Sasaki, A., Yamamoto, J., Kinjo, M., & Noda, N. (2018). Absolute Quantification of RNA Molecules Using Fluorescence Correlation Spectroscopy with Certified Reference Materials. Analytical chemistry, 90(18), 10865-10871. ‏
  2. Al-Shahib, Muhammad Baqir Sahib, Al-Saadi, Ali Hammoud, Zaidan, Haider Kamel. (2013). Principles of Molecular Genetics. Ministry of Higher Education and Scientific Research. Iraq.
  3. Rodriguez, A., Duyvejonck, H., Van Belleghem, J. D., Gryp, T., Van Simaey, L., Vermeulen, S., Mechelen, E., Vaneechoutte, M. (2020). Comparison of procedures for RNA-extraction from peripheral blood mononuclear cells. PloS one, 15(2), e0229423. ‏
  4. Cech, T. R. & Steitz, J. A. (2014). The noncoding RNA revolution-trashing old rules to forge new ones. Cell 157, 77–94.
  5. Jeon, K., Lee, J., Lee, J. S., Kim, M., Kim, H. S., Kang, H. J., & Lee, Y. K. (2019). Quantification of Cell-Free DNA: A Comparative Study of Three Different Methods. Journal of Laboratory Medicine and Quality Assurance, 41(4), 214-219. ‏
  6. Dittmar, K. A., Goodenbour, J. M., & Pan, T. (2006). Tissue-specific differences in human transfer RNA expression. PLoS genetics, 2(12), e221. ‏
  7. Chan, K. K., Kwok, C. S. N., Sze, E. T. P., & Lee, F. W. F. (2018). Evaluation of the use of TRIzol-based protein extraction approach for gel-based proteomic analysis of dried seafood products and chinese tonic foods. International journal of molecular sciences, 19(7), 1998. ‏
  8. Li, Y., Zheng, Q., Bao, C., Li, S., Guo, W., Zhao, J., ... & Huang, S. (2015). Circular RNA is enriched and stable in exosomes: a promising biomarker for cancer diagnosis. Cell research, 25(8), 981-984. ‏
  9. Lin, X., Lo, H. C., Wong, D. T., & Xiao, X. (2015). Noncoding RNAs in human saliva as potential disease biomarkers. Frontiers in genetics, 6, 175. ‏
  10. Mustafa, Nashat Ghalib. (2018). Molecular Biology. University Book House. University of Al Mosul.
  11. Carninci, P., Shibata, Y., Hayatsu, N., Itoh, M., Shiraki, T., Hirozane, T., ... & Hayashizaki, Y. (2001). Balanced-size and long-size cloning of full-length, cap-trapped cDNAs into vectors of the novel λ-FLC family allows enhanced gene discovery rate and functional analysis. Genomics, 77(1-2), 79-90. ‏
  12. Chomczynski, P., & Sacchi, N. (2006). The single-step method of RNA isolation by acid guanidinium thiocyanate–phenol–chloroform extraction: twenty-something years on. Nature protocols, 1(2), 581-585. ‏
  13. Salzman, J., Chen, R. E., Olsen, M. N., Wang, P. L. & Brown, P. O. (2013). Cell-type specific features of circular RNA expression. PLoS Genet. 9, e1003777.
  14. Sulthana, S., Basturea, G. N., & Deutscher, M. P. (2016). Elucidation of pathways of ribosomal RNA degradation: an essential role for RNase E. Rna, 22(8), 1163-1171. ‏
  15. Sharma, D., Golla, N., Singh, S., Singh, P. K., Singh, D., & Onteru, S. K. (2019). An efficient method for extracting next‐generation sequencing quality RNA from liver tissue of recalcitrant animal species. Journal of cellular physiology, 234(9), 14405-14412. ‏
  16. Peirson, S. N., & Butler, J. N. (2007). RNA extraction from mammalian tissues. In Circadian Rhythms (pp. 315-327). Humana Press. ‏
  17. Tamarin, Roberth. (2001). Principles of Genetics, Seventh Edition. The McGraw−Hill Companies. Inc. Lowell, Massachusetts.
  18. You, X., Vlatkovic, I., Babic, A., Will, T., Epstein, I., Tushev, G., ... & Chen, W. (2015). Neural circular RNAs are derived from synaptic genes and regulated by development and plasticity. Nature neuroscience, 18(4), 603-610. ‏
  19. Zhao, Z., Li, X., Gao, C., Jian, D., Hao, P., Rao, L., & Li, M. (2017). Peripheral blood circular RNA hsa_circ_0124644 can be used as a diagnostic biomarker of coronary artery disease. Scientific reports, 7(1), 1-9.
Tikrit Journal for Agricultural Sciences
Volume 21, Issue 3 - Serial Number 3
September 2021
Pages 82-89
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