We are trying to label a gene of interest with a fluorescent protein do we need to serial dilute cells for analysis?
This question is part of the following Ask The Expert session:
Choosing the Right Genome Editing Technology for your Application and Research
Answered by:
Answer
If the fluorescent tagged gene is constitutively expressed then following knock-in experiments you can enrich cells that express the fluorescent marker. Following enrichment to get a pure clonal population you can serially dilute to get single cell derived clones.