Method for the Isolation of "RNA-seq-Quality" RNA from Human Intervertebral Discs after Mortar and Pestle Homogenization

Cells. 2022 Nov 11;11(22):3578. doi: 10.3390/cells11223578.

Abstract

The problem of isolating high-quality total RNA from intervertebral discs has no recognized solution yet. This is due to the extremely low content of live cells in the samples and the voluminous intercellular matrix. A variety of published protocols focused on isolating RNA from articular cartilage have recommended the use of expensive equipment, enzymatic matrix cleavage, or cell culture. In our study, we used a combination of the traditional QIAzol protocol (Qiagen, Germany) and RNEasy column purification (Qiagen, Germany) to obtain high-quality RNA from post-surgical intervertebral disc fragments. Only a mortar and a pestle were used for grinding, making our method particularly accessible. The isolated RNA with a RIN of ~7 is suitable for studying the expression profile of chondrocytes in situ. RNA-seq analysis of three samples demonstrated cell type ratios to be mostly relevant to intervertebral disc tissues, with over 70% of the chondrocytes of the three subtypes having an admixture of blood-related cells.

Keywords: RIN; RNA-seq; cartilage RNA isolation; intervertebral disc.

Publication types

  • Research Support, Non-U.S. Gov't

MeSH terms

  • Cartilage, Articular* / metabolism
  • Chondrocytes / metabolism
  • Humans
  • Intervertebral Disc*
  • RNA / metabolism
  • RNA-Seq

Substances

  • RNA

Grants and funding

This work was supported by the Russian Science Foundation (RSF) grant No. 22-15-20037 and by the Government of the Novosibirsk region.