Hi all,
I made a mistake for the first time during my 7 years of cell culture and I have no idea what I should do. So I just made a fresh cell culture media stock in the original bottle (Gibco DMEM + 10% FBS +1% Pen-strap). Then I use this stock to subculture cells and plate them in petri dishes as usually. However, I wasn't focus enough and I accidently use a pipette tip that has contacted diluted cells to transfer fresh media from the stock bottle. You can imagine there are cells attached to the wall inside the pipette tip and now they are floating in my 500ml fresh stock. I took out 3ml from the contaminated media and plate in a petri dish to test if they will grow. I will be using the media for the same cell line all the time. Should I throw it away? Or I can still use it on the same cell line? Since its worth over 60 dollars (cause it has 50ml FBS in it), I hope I can still use it.
Any idea is appreciated!