Pipetting
Adapted from Lotterhos Lab pipetting protocol.
Pipettes in the Lab
Single channels:
P2.5 (.1-2.5 uL)
P10 (.5-10 uL)
P20 (2-20 uL)
P100 (10-100 uL)
P200 (20-200 uL)
P1000 (100-1000 uL)
Multichannels:
P10 (.5-10 uL)
P100 (10-100 uL)
p1200 (120-1200 uL)
Electronic Single Channels
P20 (1-20 uL)
P100 (5-100 uL)
P1000 (50-1000 uL)
Electronic Multi Channels
P10 (0.5-10 uL)
P100 (5-100 uL)
P1200 (50-1200 uL)
Filtered vs. Non-Filtered Pipette Tips
All pipettes in the lab have both filtered and non-filtered compatible tips.
Filtered tips help prevent whatever you’re pipetting from getting into the pipette through aspiration. Therefore, it is best to use filtered tips when working with different samples to prevent cross contamination from any sample that has gotten into the pipette (ex. when pipetting different DNA samples for a DNA extraction)
Unfiltered tips are appropriate to use when pipetting solutions, dyes, and buffers, i.e. things less likely to cause significant contamination to other pipetted materials. (Ex. loading dye, gel ladders, extraction buffers, etc.)
Spray a kimwipe with ethanol and wipe down pipettes before and after use to remove any potential remaining sample.
Pointers for Pipetting
Drawing up liquid. Check the amount on the pipette is correct. When pipetting, be sure only to push down on the plunger to the first stop and slowly release to pick up the liquid until your thumb comes completely off the plunger. If you go past the first stop, you will draw up more liquid than the amount you set on the pipette and/or create bubbles. If you push down and then release quickly to draw up liquid, it can cause aspiration and contaminate the pipette if you aren’t using filtered tips. If you are using filtered tips, aspiration can cause liquid to land on the filter, so the pipette tip will hold less liquid than you specified. When drawing up liquid, you may choose to pipette up and down 3 times to pre-wet the pipette tip. Ensure to only go to the first stop for each of the 3 times.
Check the pipette tip has the correct amount. Look at the pipette tip, or all the pipette tips if using the multichannel. Does it have the amount of liquid that you expect? Are there air bubbles (other than a tiny bubble that often forms at the very apex of the tip)? If so, push out the liquid and restart.
Pushing out liquid. Slowly push down on the plunger past the first stop until you reach the final stopping point for the plunger. Keep your thumb on the plunger until the tip of the pipette is completely removed from the solution. Drawing up your thumb before the tip is removed will suck up some of the solution.
Check the pipette tip is empty. After you push the liquid out, check the pipette tip again and make sure it is empty. Dispose of the tip in a EHS-labeled waste jar. If there is any liquid in the tip that didn’t get pushed out or beads of liquid on the inside of the tip, proceed to the next step.
Solution is stuck in the pipette tip. If there is any liquid in the tip that didn’t get pushed out, carefully take the tip off. When you put the tip back on the pipette, some of the liquid may get pushed out, so carefully put the tip back on over the well where the solution needs to go. Then push down to the second stop and push the rest of the liquid out.