Having difficulties with your experiment?

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View the relevant questions below:

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Getting Started page

General

Why have my primary cells started to slow in growth or stopped growing?

Primary cells are not immortalized and undergo a limited number of population doublings. Each cell type has a different maximum population doubling number that is found on the certificate of analysis for the assigned lot number. For information on “Population Doubling” vs. “Passage Number” refer to the “Getting Started”  page.

Why aren’t my cells attaching to the surface of the plate/flask?

Be sure to use the Coating Matrix Kit if you are using the Animal Origin–Free (AOF) supplementation for your culture. There are no attachment factors in the AOF supplements, and Coating Matrix Kit is required for cells to adhere properly.

Can I transfect my primary cells?

Yes, we strongly recommended that you contact our Molecular Biology scientists at techsupport@thermofisher.com to help you choose the best transfection reagent option, as primary cells tend to be very sensitive.

Why do I have such low viability of my primary cells upon thaw?

It is important to store the cells, once received, in the vapor phase of liquid nitrogen. The vials are not leak proof, and submerging them into the liquid phase can allow liquid nitrogen to leak into the vial and affect the viability of the cells.

I see large, flat pancake-looking cells in my keratinocyte culture. What are they?

These are senescent cells, and this is normal for adult keratinocyte culture. You always have a population of cells that are old and no longer proliferate. However younger cells, which are small in size should keep proliferating. When a culture gets older, you see more and more large cells, and the culture will eventually stop growing. With the right care an attention, the culture should yield at least 25 population doublings. 

I thawed my keratinocyte cells and just plated them into a few flasks/plates and I’m seeing a lot of floating cells. Why is this?

It is very important to do a viability count prior to plating and to follow the recommended seeding density. The flask number mentioned in some of the protocols is a guideline so that you are aware of how many vessels should be anticipated from each vial. Cell counts on the vial are the minimum guaranteed, but there are usually more supplied to make sure that you receive the amount of cells that we promise. That being said, it is important to count the cells to make sure you have the correct seeding density and so that you can monitor the number of population doublings that your cells go through. 

Hepatocytes
I’m getting low post-thaw cell viability with my hepatocytes. What should I do?

Please see the following causes and recommendations:

Possible cause

Recommendation

Improper thawing technique

  • Review thawing, plating and counting protocols
  • Thaw cells <2 mins at 37 degrees C
Sub-optimal thawing mediumUse HTM Medium during thawing to remove cryoprotectant
Rough handling of hepatocytes during counting
  • Mix slowly, use wide-bore pipette tips
  • Ensure a homogenous cell mixture prior to counting

Improper counting technique

  • Count cells on 2 of the 4 grid lines
  • Do not let cells sit in trypan blue mixture for more than 1 min prior to loading

Cells left out too long

Plate cells immediately after counting

For additional information, please refer to the ADME/Tox Support Center.

I’m getting an unexpectedly low hepatocyte yield. What could be the cause of this?

Please see the following causes and recommendations:

Possible cause

Recommendation

Improper thawing technique

  • Review thawing, plating and counting protocols
  • Thaw cells <2 mins at 37 degrees C
Sub-optimal thawing mediumUse HTM Medium during thawing to remove cryoprotectant
Incorrect centrifugation speedCheck thawing protocol for proper centrifugation speed and time (varies by species; human is 100 x g for 10 min at RT)

Rough handling of hepatocytes during counting

  • Mix slowly, use wide-bore pipette tips
  • Ensure a homogenous cell mixture prior to counting

Improper counting technique

  • Count cells on 2 of the 4 grid lines
  • Do not let cells sit in trypan blue mixture for more than 1 min prior to loading

For additional information, please refer to the ADME/Tox Support Center.

I’m getting low attachment efficiency with my hepatocytes. What should I do?

Please see the following causes and recommendations:

Possible cause

Recommendation
Not enough time for cells to attach
  • Wait before overlaying with Geltrex Matrix to see if attachment increases
  • Compare cultures to pictures on the lot-specific characterization specification sheet (human cells)
Poor-quality substratumUse Gibco Collagen I-Coated Plates
Hepatocyte lot not characterized as plateable
  • Check lot specifications to ensure it is qualified for plating
  • Review thawing, plating, and counting protocols

For additional information, please refer to the ADME/Tox Support Center.

I have a sub-optimal monolayer confluency for my hepatocytes. What should I do?

Please see our recommendations above for:

Possible cause

Recommendation

Seeding density too low

Check lot-specific characterization specification sheet for appropriate seeding density (human cells)  Observe cells under microscope for appropriate seeding prior to incubation

Insufficient dispersion of hepatocytes during plating

Disperse cells evenly by moving plate slowly in a figure-eight and back and forth pattern in incubator

Insufficient plating volume used for well format

Refer to literature or technical support for suggested plating volumes

Low attachment efficiency

Please see our recommendations above for: “I’m getting low attachment efficiency with my hepatocytes. What should I do?”

Some animal lots are not >80% confluent

Check lot-specific characterization specification sheet for appropriate seeding density.  Note: Some animal species create chains or islands of cells rather than being 100% confluent.

For additional information, please refer to the ADME/Tox Support Center.

I am seeing rounded up cell clumps or debris on top of the hepatocyte monolayer. What should I do?

Please see the following causes and recommendations:

Possible cause

Recommendation
Seeding density too high
  • Check lot-specific characterization specification sheet for appropriate seeding density (human cells)
  • Observe cells under microscope for appropriate seeding prior to incubation
Insufficient dispersion of hepatocytes during plating
  • Disperse cells evenly by moving plate slowly in a figure-eight and back-and-forth pattern in incubator
  • Shake plate and wash cell monolayers prior to applying Geltrex Matrix overlay
Improper plating volume used for well formatRefer to literature or technical support for suggested plating volumes

For additional information, please refer to the ADME/Tox Support Center.

I’m getting a loss of membrane integrity or cuboidal cell shape with my hepatocytes. What should I do?

Please see the following causes and recommendations:

Possible cause

Recommendation
Hepatocyte lot not characterized as plateableCheck lot specifications to ensure it is qualified for plating

Sub-optimal culture medium

  • Williams Medium E with Plating and Incubation Supplement Packs
  • Refer to our plating protocol
Cells were cultured for too longIn general, plateable cryopreserved hepatocytes should not be cultured for more than five days

For additional information, please refer to the ADME/Tox Support Center.

I’m seeing sub-optimal bile canlicular formation with my hepatocytes. What should I do?

Please see the following causes and recommendations:

Possible cause

Recommendation
Hepatocyte lot not transporter-qualifiedCheck lot specifications to ensure it is transporter-qualified

Sub-optimal culture medium

  • Use Williams Medium E with Plating and Incubation Supplement Packs
  • Refer to our plating protocol
Not enough time for bile canaliculi to formIn general, at least 4–5 days in culture is required for bile canalicular network formation

For additional information, please refer to the ADME/Tox Support Center.

I’m getting unexpected induction results with my hepatocytes. What could be causing this?

First of all, we recommend comparing results to those reported on our lot-specific characterization specification sheet (human cells) and also referring to our enzyme induction protocol. Here are other potential causes and recommendations:

Possible Cause

Recommendation

Sub-optimal monolayer confluency

 

Please see our recommendations above for ‘I have a sub-optimal monolayer confluency for my hepatocytes. What should I do?’

Poor monolayer integrity

 

Please see our recommendations below for ‘With my hepatocytes, I’m seeing rounding up of the cells, cellular debris, and/or holes in the monolayer, indicating dying cells. What should I do?’
Inappropriate positive control

Check positive control to ensure suitability

Incorrect concentration of positive control

Use the correct concentration of positive control

For additional information, please refer to the ADME/Tox Support Center.

With my hepatocytes, I’m seeing rounding up of the cells, cellular debris, and/or holes in the monolayer, indicating dying cells. What should I do?

This could be due to the toxicity of the test compound. Here are other potential causes and recommendations:

Possible cause

Recommendation
Sub-optimal culture medium
  • Use Williams Medium E with Plating and Incubation Supplement Packs
  • Refer to our plating protocol
Hepatocyte lot not characterized as plateableCheck lot specifications to ensure it is qualified for plating

Cells were cultured for too long

In general, plateable cryopreserved hepatocytes should not be cultured for more than five days

For additional information, please refer to the ADME/Tox Support Center.

Neural Cells
Why did my neuron cells form clumps when I seeded them onto a 96-well plate, but not into large flasks?

There are two possible causes for this issue:

  • It is more likely that the matrix coated on the 96-well plate dried because the time interval between removal of coating solution and addition of cells was too long. Once the coating matrix is dry, the cells likely lose the attachment ability. We recommend shortening the interval between removal of coating solution and addition of cells, and work with only a few wells at a time.
  • It takes more time to dispense cells in a 96-well plate so that the remaining cells in the tube could form clumps. We recommend that you resuspend the cells well before dispensing them.
Why are there no viable primary neuron cells/astrocytes/rat glial precursor cells after thawing the cell stock?

These cells are very fragile. We recommend that you follow the procedure in the manual and use the correct medium. Fast thawing is the key for healthy culture. There are several critical points to consider:

  • Pre-rinse all materials with medium before use. Do not use PBS, DPBS, or HBSS to rinse because they do not contain proteins.
  • Thaw cells quickly and do not expose cells to air. 
  • Transfer cells to a pre-rinsed tube first, then add slowly add medium in a drop-wise manner. Do not add the full amount of medium to the cells at once because this may lead to decreased cell viability due to osmotic shock.
  • Use pre-warmed complete growth medium and correct seeding density. 
  • Matrix coating is required for some cell cultures.
  • For primary neuron cells, do not centrifuge the cells as they are extremely fragile upon recovery from cryopreservation.
Why did my Gibco™ PSC Neural Induction Medium (Cat. No. A1647801) fail to induce neural stem cells?

There are several possibilities causing the failure of neural induction:

  • High quality of hPSC cells is critical to the success of neural induction. Remove differentiated and partially differentiated hPSC cells before neural induction.
  • Before plating hPSCs for induction, cell counting is recommended because too low or too high cell confluency will reduce induction efficiency. The recommended plating density for induction is 2–2.5 x 10E4cells/cm2.
  • Cell clumps but not single cell suspension should be plated for induction.
  • To increase induction efficiency, overnight treatment with 10 µM ROCK Inhibitor Y27632 at the time hPSC splitting can be used to prevent extensive cell death.
Why did my Gibco™ B-27™ Supplement have poor performance?
  • Check if the correct B-27™ Supplement was used to culture the cells.
  • Check expiration date of B-27™ Supplement to see if it has expired.
  • Check if the B-27™ supplemented medium used was fresh. The supplemented medium is stable for only 2 weeks at 4°C. 
  • Check if the B-27™ Supplement was exposed to excessive heat. Thawed B-27™ Supplement should not be exposed to RT or higher for more than 30 mins. 
  • Check if the B-27™ supplement was thawed and refrozen multiple times. Thawed B-27™ Supplement at 4°C should be used within 1 week.
  • Check appearance of the B-27™ Supplement. It should be a transparent yellow liquid. Green color appearance indicates that the supplement is not good.

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