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Single-cell genomics technologies are currently in full swing, such as single-cell RNA sequencing (scRNA-seq) and chromatin transposase accessibility sequencing (ATAC-seq)
In this process, we must accurately count the nuclei
Compared with traditional large-volume cell sequencing methods, single-cell genomics technology highlights the differences between cells and helps to gain a deeper understanding of sample materials
However, such studies require accurate counting of isolated nuclei, because the requirements for library preparation are the minimum number of unlysed cells, and the sample does not contain cell clumps and debris
AO/PI staining is more reliable than trypan blue
People usually use cell viability indicators to count the isolated nuclei
For this reason, acridine orange/propidium iodide (AO/PI) staining is the first choice, whether for routine cell viability testing or single-cell genomics research
This method has also recently been applied to single-cell genomics applications, where green corresponds to intact cells and red corresponds to successfully isolated nuclei
Fully automated cell counting
For samples stained with AO/PI, we can manually evaluate the staining results under a fluorescence microscope
At the same time, when selecting an automatic cell counter for single-cell genomics research, in addition to the fluorescence counting capability, the need for the sample size of the instrument should also be considered
In addition, when dealing with challenging samples, such as tissue lysates, the advantages of AO/PI staining over trypan blue are more obvious
Researchers have used an automatic cell counter to count cell nuclei isolated from mouse brains and compared the two methods
There are many fluorescence cell counters on the market, such as the CellDrop fluorescence/bright field cell counter