Method for isolating and purifying RNA from biological materials

摘要

Includes the following steps: (1) Mix organs and tissues with formamide and monovalent cation salt solution, homogenize them to obtain the dehydrated biological sample; (2) Mix the dehydrated biological sample with monovalent cation salt solution for incubation; (3) Add the monovalent cation salt solution with precipitation effect to the mixture, mix them and centrifuge, then pour the supernatant into another centrifuge tube; (4) Add isopropanol, mix it and centrifuge, and then discard the upper phase liquid, the lower phase liquid and the visible residual impurities between the upper and lower phases to get white RNA precipitate. This method proposed in the invention enables efficient isolation of protein from RNA in the biological samples. It avoids decomposition of RNA by the residual protein that remains in the products; the reagent used in the invention is low-toxicity compound with little hazard to the environment and human body; since the products obtained are not easily decomposed, the products can be transported at long distance and stored at room temperature; the method is easy to operate and no special skill is required for the operator. The equipment used is simple and cost efficient and enables high RNA yield and high purity.

主权项

1. A method for isolating and purifying RNA from biological materials comprising the following steps:
(1) preparing a dehydrated biological sample by either adding tissues and organs to a mixture between formamide and 3M-13.5M monovalent cation salt solution at volume ratio greater than 1 and homogenizing the mixture for 5 seconds to 20 minutes to obtain a dehydrated biological sample; wherein the ratio between the tissues and organs and the mixture is between 05 mg:1 ml and 200 mg:1 ml and the tissues and organs are from animals, plants, or fungi; or adding a single-cell precipitate to the mixture between formamide and monovalent cation salt solution at a volume ratio greater than 1, suspending the precipitate at 0˜25° C. or homogenizing it at 0˜37° C. for 20 seconds to 20 minutes to obtain a dehydrated biological sample; wherein the single cell precipitate is obtained from cultured Gram positive bacteria cells, Gram negative bacteria cells, or fungi cells, cultured cells of animal or plant cells, blood cells or sperm cells; (2) mixing the dehydrated biological sample with 3M-13.5M monovalent cation salt solution at a volume ratio greater than 1, or mixing the dehydrated biological sample with 3M-13.5M monovalent cation salt solution and Formamide solution containing sodium dodecyl sulfate of a mass concentration of 5%-40% at a volume ratio of 160:50:40, incubating the resulting mixture at 0˜95° C. for 0.5˜120 min, and leaving it alone at 0˜40° C. for 0˜10 min; (3) adding 3.3M-5M monovalent cation salt solution to the mixture obtained in step (2) at a volume ratio between 200:1000 and 400:1000 mixing the resulting mixture, centrifuging it in a centrifuge tube for 0.15˜30 min at 2000˜16000 g at 4˜25° C., and then pouring the supernatant into another centrifuge tube; (4) adding isopropanol to the supernatant at a volume ratio between 900:300 and 900:800, mixing, centrifuging in a centrifuge tube for 1˜30 min at 2000˜16000 g at 4˜37° C., and then discarding the upper phase liquid, the lower phase liquid and the visible residual solid impurity between the upper and lower phases to get a white RNA precipitate at the bottom of the centrifuge tube.