Difference: ProtocolsFreezingStrains (1 vs. 9)

Revision 92024-02-03 - JeffreyBarrick

 
META TOPICPARENT name="ProtocolList"

Freezing Strains

Supplies

  1. Overnight liquid culture
    Several milliliters of overnight liquid culture grown in a suitable medium for each sample to be frozen.
  2. 80% Glycerol or DMSO solution
    A standard lab solution. Grab your own stock bottle and keep it in your workspace.
  3. Sterile 2 ml cryovials
    Take a bag for yourself and keep it in your workspace, closing it with an alligator clip when not in use.
  4. Cryotag rectangular 1.28" x 0.50" labels
    Found in the office supplies.
  5. Clear tape
    Found in dispensers throughout lab. Do NOT use "magic" tape (which is translucent and does not stick as well at –80°C). Use fully clear tape.
  6. Freezer box
    With 81 tube insert (9 × 9 grid).

Labeling Cryovials


Materials for labeling a cryovial and closeup of properly labeled vial
  1. Sample naming – Every strain has a three letter designation (usually the initials of someone) and a strain number. When freezing new samples, either append them to your own strain series or obtain the next available numbers from a standard series (e.g. JEB) by looking in the Strain Database.
  2. Write the three letter designation, the strain number, and the date (MM–DD–YY) along with whatever other distinctive information about the strain that can be fit onto the label (e.g. experiment, population, time) on a CRYOTAG label for each sample. You can find the templates for these special stickers below, and, 'Rectangle_ToughSpot.doc' is most often used. Find the special labels to print on in Lab A under where the FedEx labels are stored. It is recommended to manually feed this paper into the printer (use the printer in Lab B), so open the manual feeder on the side of the printer, place it face down, and ensure that the correct tray (Tray 1, manual) is listed when you click 'print.'
  3. Stick the label on tube horizontally, and completely cover it with one strip of clear tape (not magic tape!) for longevity.
  4. Write the strain number on the plastic circular cap insert, so that it will be visible from above when looking down on the tube in a freezer box.

Labeling Freezer Boxes


Example of a labeled freezer box
  1. Box Naming - Every box should be labeled with your last name and a number. Use this system and not a special name for each box.
  2. Print out two copies of your labels with the Dymo labeler. One should have your last name and one should have "Box X" on it.
  3. Place the labels on both the bottom and lid of your box. Do this on a dry and room-temperature box so that they will stick. Do not do it on one that you have already had in the freezer!
  4. Completely cover labels in clear packing tape for longevity.

Freezing Samples

Changed:
<
<		You will need to add a cryoprotectant to your sample of cells to be frozen. Generally this is 80% glycerol, though for some experiments DMSO is used instead. The standard amount to add of this cryoprotectant is one-fifth the volume of your cells. This gives a final concentration of 13.3% glycerol or 16.7% DMSO.
>
>		You will need to add a cryoprotectant to your sample of cells to be frozen. Generally we use a sterilized 80% (v/v) glycerol stock because, while still viscous, this is much easier to pipette than 100% glycerol. For some type of cells 100% DMSO is used instead. A standard final concentration of cryoprotectant is in the 10-20% (v/v) range. Typically, we add one volume of cryoprotectant stock solution per five times that volume of culture. This gives a final concentration of 13.3% (v/v) glycerol if using the 80% (v/v) stock or 16.7% (v/v) DMSO.
  If you are using DMSO, wear gloves and avoid contact with your skin!

For most samples, you can follow this procedure:

Changed:
<
<		 1 Add 200 µl of 80% glycerol to each empty cryovial. Glycerol is extremely viscous. Use the 1 ml pipettor because the tips have a larger aperture. Be careful to pull liquid into the pipette tip slowly and to let excess liquid drip off the outside before you remove the tip from the stock bottle. Use the repeat pipettor if you are freezing >12 samples.
>
>
  1. Add 200 µl of 80% glycerol to each empty cryovial. Glycerol is extremely viscous. Use the 1 ml pipettor because the tips have a larger aperture. Be careful to pull liquid into the pipette tip slowly and to let excess liquid drip off the outside before you remove the tip from the stock bottle. Use the repeat pipettor if you are freezing >12 samples.
 
  1. Add 1000 µl of each revived strain to the appropriately labeled cryovial using a 1 ml pipettor.
  2. Vortex each cryovial at high speed to be sure that these solutions are uniformly mixed.
  3. Place the tubes in the next positions available in your boxes or the main lab stock boxes. Record the box, rack, and freezer names and numbers.

Updating the Strain Database

It is very important to immediately add information about the samples you have archived to the lab database so that they can be located by others and posterity. You should also keep a record in your lab notebook of where these samples came from. Instructions for how to use the strain database are located here:

External site Strain Database Instructions

External site Label Templates

Additional information for strains from ATCC

Strains from ATCC typically arrive as freeze-dried samples. After you break the vial, you should resuspend the cells in a ~400 µl of the media suggested by ATCC for growth of your strain. Because these are type strains and we don't want to accidentally select a mutant as our version of the type strain, we archive the following samples:

  • Mixed Population: Immediately add ~100 µl of the resuspension (~1/4 of the total volume) to liquid media. This outgrowth will be the original "mixed population" sample.
  • Clonal Isolates: Streak out from the remainder of the resuspension on a suitable agar plate. Grow as directed, pick 3 colonies to grow in liquid media, and archive as c1, c2, c3. These are the "clonal isolate" samples. The c1 sample will be the one that you use in your experiments and check genetically and phenotypically to be sure it is the correct strain, and not a mutant or contamination!
  • Freeze-Dried: Freeze the remainder of the original resuspension of the freeze-dried culture at –80°C using 10-20% DMSO as cryoprotectant. This is the "original freeze-dried stock".

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Revision 82019-04-09 - SarahBialik

 
META TOPICPARENT name="ProtocolList"

Freezing Strains

Supplies

  1. Overnight liquid culture
    Several milliliters of overnight liquid culture grown in a suitable medium for each sample to be frozen.
  2. 80% Glycerol or DMSO solution
    A standard lab solution. Grab your own stock bottle and keep it in your workspace.
  3. Sterile 2 ml cryovials
    Take a bag for yourself and keep it in your workspace, closing it with an alligator clip when not in use.
  4. Cryotag rectangular 1.28" x 0.50" labels
    Found in the office supplies.
  5. Clear tape
    Found in dispensers throughout lab. Do NOT use "magic" tape (which is translucent and does not stick as well at –80°C). Use fully clear tape.
  6. Freezer box
    With 81 tube insert (9 × 9 grid).

Labeling Cryovials


Materials for labeling a cryovial and closeup of properly labeled vial
  1. Sample naming – Every strain has a three letter designation (usually the initials of someone) and a strain number. When freezing new samples, either append them to your own strain series or obtain the next available numbers from a standard series (e.g. JEB) by looking in the Strain Database.
Changed:
<
<
  1. Write the three letter designation, the strain number, and the date (MM–DD–YY) on a CRYOTAG label for each sample. Also include whatever other distinctive information about the strain that can be fit onto the label (e.g. experiment, population, time).
  2. Stick the label on tube horizontally, and completely cover it with one strip of clear tape for longevity.
>
>
  1. Write the three letter designation, the strain number, and the date (MM–DD–YY) along with whatever other distinctive information about the strain that can be fit onto the label (e.g. experiment, population, time) on a CRYOTAG label for each sample. You can find the templates for these special stickers below, and, 'Rectangle_ToughSpot.doc' is most often used. Find the special labels to print on in Lab A under where the FedEx labels are stored. It is recommended to manually feed this paper into the printer (use the printer in Lab B), so open the manual feeder on the side of the printer, place it face down, and ensure that the correct tray (Tray 1, manual) is listed when you click 'print.'
  2. Stick the label on tube horizontally, and completely cover it with one strip of clear tape (not magic tape!) for longevity.
 
  1. Write the strain number on the plastic circular cap insert, so that it will be visible from above when looking down on the tube in a freezer box.

Labeling Freezer Boxes


Example of a labeled freezer box
  1. Box Naming - Every box should be labeled with your last name and a number. Use this system and not a special name for each box.
  2. Print out two copies of your labels with the Dymo labeler. One should have your last name and one should have "Box X" on it.
  3. Place the labels on both the bottom and lid of your box. Do this on a dry and room-temperature box so that they will stick. Do not do it on one that you have already had in the freezer!
  4. Completely cover labels in clear packing tape for longevity.

Freezing Samples

You will need to add a cryoprotectant to your sample of cells to be frozen. Generally this is 80% glycerol, though for some experiments DMSO is used instead. The standard amount to add of this cryoprotectant is one-fifth the volume of your cells. This gives a final concentration of 13.3% glycerol or 16.7% DMSO.

If you are using DMSO, wear gloves and avoid contact with your skin!

For most samples, you can follow this procedure:

1 Add 200 µl of 80% glycerol to each empty cryovial. Glycerol is extremely viscous. Use the 1 ml pipettor because the tips have a larger aperture. Be careful to pull liquid into the pipette tip slowly and to let excess liquid drip off the outside before you remove the tip from the stock bottle. Use the repeat pipettor if you are freezing >12 samples.

  1. Add 1000 µl of each revived strain to the appropriately labeled cryovial using a 1 ml pipettor.
  2. Vortex each cryovial at high speed to be sure that these solutions are uniformly mixed.
  3. Place the tubes in the next positions available in your boxes or the main lab stock boxes. Record the box, rack, and freezer names and numbers.

Updating the Strain Database

It is very important to immediately add information about the samples you have archived to the lab database so that they can be located by others and posterity. You should also keep a record in your lab notebook of where these samples came from. Instructions for how to use the strain database are located here:

External site Strain Database Instructions

External site Label Templates

Additional information for strains from ATCC

Strains from ATCC typically arrive as freeze-dried samples. After you break the vial, you should resuspend the cells in a ~400 µl of the media suggested by ATCC for growth of your strain. Because these are type strains and we don't want to accidentally select a mutant as our version of the type strain, we archive the following samples:

  • Mixed Population: Immediately add ~100 µl of the resuspension (~1/4 of the total volume) to liquid media. This outgrowth will be the original "mixed population" sample.
  • Clonal Isolates: Streak out from the remainder of the resuspension on a suitable agar plate. Grow as directed, pick 3 colonies to grow in liquid media, and archive as c1, c2, c3. These are the "clonal isolate" samples. The c1 sample will be the one that you use in your experiments and check genetically and phenotypically to be sure it is the correct strain, and not a mutant or contamination!
  • Freeze-Dried: Freeze the remainder of the original resuspension of the freeze-dried culture at –80°C using 10-20% DMSO as cryoprotectant. This is the "original freeze-dried stock".

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Revision 72016-12-15 - JeffreyBarrick

 
META TOPICPARENT name="ProtocolList"

Freezing Strains

Supplies

  1. Overnight liquid culture
    Several milliliters of overnight liquid culture grown in a suitable medium for each sample to be frozen.
  2. 80% Glycerol or DMSO solution
    A standard lab solution. Grab your own stock bottle and keep it in your workspace.
  3. Sterile 2 ml cryovials
    Take a bag for yourself and keep it in your workspace, closing it with an alligator clip when not in use.
  4. Cryotag rectangular 1.28" x 0.50" labels
    Found in the office supplies.
  5. Clear tape
    Found in dispensers throughout lab. Do NOT use "magic" tape (which is translucent and does not stick as well at –80°C). Use fully clear tape.
Changed:
<
<
  1. Freezer box
    With 81 tube insert (9 &multiply; 9 grid).
>
>
  1. Freezer box
    With 81 tube insert (9 × 9 grid).
 

Labeling Cryovials


Materials for labeling a cryovial and closeup of properly labeled vial
  1. Sample naming – Every strain has a three letter designation (usually the initials of someone) and a strain number. When freezing new samples, either append them to your own strain series or obtain the next available numbers from a standard series (e.g. JEB) by looking in the Strain Database.
  2. Write the three letter designation, the strain number, and the date (MM–DD–YY) on a CRYOTAG label for each sample. Also include whatever other distinctive information about the strain that can be fit onto the label (e.g. experiment, population, time).
  3. Stick the label on tube horizontally, and completely cover it with one strip of clear tape for longevity.
  4. Write the strain number on the plastic circular cap insert, so that it will be visible from above when looking down on the tube in a freezer box.

Labeling Freezer Boxes


Example of a labeled freezer box
  1. Box Naming - Every box should be labeled with your last name and a number. Use this system and not a special name for each box.
  2. Print out two copies of your labels with the Dymo labeler. One should have your last name and one should have "Box X" on it.
  3. Place the labels on both the bottom and lid of your box. Do this on a dry and room-temperature box so that they will stick. Do not do it on one that you have already had in the freezer!
  4. Completely cover labels in clear packing tape for longevity.

Freezing Samples

You will need to add a cryoprotectant to your sample of cells to be frozen. Generally this is 80% glycerol, though for some experiments DMSO is used instead. The standard amount to add of this cryoprotectant is one-fifth the volume of your cells. This gives a final concentration of 13.3% glycerol or 16.7% DMSO.

If you are using DMSO, wear gloves and avoid contact with your skin!

For most samples, you can follow this procedure:

Changed:
<
<		 1 Add 200uL of 80% glycerol to each empty cryovial. Glycerol is extremely viscous. Use the 1 ml pipettor because the tips have a larger aperture. Be careful to pull liquid into the pipette tip slowly and to let excess liquid drip off the outside before you remove the tip from the stock bottle. Use the repeat pipettor if you are freezing >12 samples.
  1. Add 1000uL of each revived strain to the appropriately labeled cryovial using a 1 ml pipettor.
>
>		 1 Add 200 µl of 80% glycerol to each empty cryovial. Glycerol is extremely viscous. Use the 1 ml pipettor because the tips have a larger aperture. Be careful to pull liquid into the pipette tip slowly and to let excess liquid drip off the outside before you remove the tip from the stock bottle. Use the repeat pipettor if you are freezing >12 samples.
  1. Add 1000 µl of each revived strain to the appropriately labeled cryovial using a 1 ml pipettor.
 
  1. Vortex each cryovial at high speed to be sure that these solutions are uniformly mixed.
  2. Place the tubes in the next positions available in your boxes or the main lab stock boxes. Record the box, rack, and freezer names and numbers.

Updating the Strain Database

It is very important to immediately add information about the samples you have archived to the lab database so that they can be located by others and posterity. You should also keep a record in your lab notebook of where these samples came from. Instructions for how to use the strain database are located here:

External site Strain Database Instructions

External site Label Templates

Additional information for strains from ATCC

Strains from ATCC typically arrive as freeze-dried samples. After you break the vial, you should resuspend the cells in a ~400 µl of the media suggested by ATCC for growth of your strain. Because these are type strains and we don't want to accidentally select a mutant as our version of the type strain, we archive the following samples:

  • Mixed Population: Immediately add ~100 µl of the resuspension (~1/4 of the total volume) to liquid media. This outgrowth will be the original "mixed population" sample.
  • Clonal Isolates: Streak out from the remainder of the resuspension on a suitable agar plate. Grow as directed, pick 3 colonies to grow in liquid media, and archive as c1, c2, c3. These are the "clonal isolate" samples. The c1 sample will be the one that you use in your experiments and check genetically and phenotypically to be sure it is the correct strain, and not a mutant or contamination!
  • Freeze-Dried: Freeze the remainder of the original resuspension of the freeze-dried culture at –80°C using 10-20% DMSO as cryoprotectant. This is the "original freeze-dried stock".

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Changed:
<
<
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>
>
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Revision 62016-04-07 - JeffreyBarrick

 
META TOPICPARENT name="ProtocolList"

Freezing Strains

Supplies

  1. Overnight liquid culture
    Several milliliters of overnight liquid culture grown in a suitable medium for each sample to be frozen.
  2. 80% Glycerol or DMSO solution
    A standard lab solution. Grab your own stock bottle and keep it in your workspace.
Changed:
<
<
  1. Sterile 2 ml cryovials and circular cap inserts
    Found on a shelf above the colony counters in 1.436. Take a bag for yourself and keep it in your workspace, closing it with an alligator clip when not in use.
  2. Cryotag rectangular 1.28" x 0.50" labels
    Found in the bottom drawer of the office supply cabinet below the message board in 1.436.
  3. Clear tape
    Found in dispensers throughout lab or on the office supply cabinet in 1.436. Do NOT use "magic" tape (which is translucent and does not stick as well at –80°C). Use fully clear tape.
  4. Freezer box
>
>
  1. Sterile 2 ml cryovials
    Take a bag for yourself and keep it in your workspace, closing it with an alligator clip when not in use.
  2. Cryotag rectangular 1.28" x 0.50" labels
    Found in the office supplies.
  3. Clear tape
    Found in dispensers throughout lab. Do NOT use "magic" tape (which is translucent and does not stick as well at –80°C). Use fully clear tape.
  4. Freezer box
    With 81 tube insert (9 &multiply; 9 grid).
 
Changed:
<
<

Labeling Tubes

>
>

Labeling Cryovials

 
Added:
>
>

Materials for labeling a cryovial and closeup of properly labeled vial
 
  1. Sample naming – Every strain has a three letter designation (usually the initials of someone) and a strain number. When freezing new samples, either append them to your own strain series or obtain the next available numbers from a standard series (e.g. JEB) by looking in the Strain Database.
  2. Write the three letter designation, the strain number, and the date (MM–DD–YY) on a CRYOTAG label for each sample. Also include whatever other distinctive information about the strain that can be fit onto the label (e.g. experiment, population, time).
  3. Stick the label on tube horizontally, and completely cover it with one strip of clear tape for longevity.
  4. Write the strain number on the plastic circular cap insert, so that it will be visible from above when looking down on the tube in a freezer box.
Added:
>
>

Labeling Freezer Boxes


Example of a labeled freezer box
  1. Box Naming - Every box should be labeled with your last name and a number. Use this system and not a special name for each box.
  2. Print out two copies of your labels with the Dymo labeler. One should have your last name and one should have "Box X" on it.
  3. Place the labels on both the bottom and lid of your box. Do this on a dry and room-temperature box so that they will stick. Do not do it on one that you have already had in the freezer!
  4. Completely cover labels in clear packing tape for longevity.
 

Freezing Samples

You will need to add a cryoprotectant to your sample of cells to be frozen. Generally this is 80% glycerol, though for some experiments DMSO is used instead. The standard amount to add of this cryoprotectant is one-fifth the volume of your cells. This gives a final concentration of 13.3% glycerol or 16.7% DMSO.

If you are using DMSO, wear gloves and avoid contact with your skin!

For most samples, you can follow this procedure:

1 Add 200uL of 80% glycerol to each empty cryovial. Glycerol is extremely viscous. Use the 1 ml pipettor because the tips have a larger aperture. Be careful to pull liquid into the pipette tip slowly and to let excess liquid drip off the outside before you remove the tip from the stock bottle. Use the repeat pipettor if you are freezing >12 samples.

  1. Add 1000uL of each revived strain to the appropriately labeled cryovial using a 1 ml pipettor.
  2. Vortex each cryovial at high speed to be sure that these solutions are uniformly mixed.
  3. Place the tubes in the next positions available in your boxes or the main lab stock boxes. Record the box, rack, and freezer names and numbers.

Updating the Strain Database

It is very important to immediately add information about the samples you have archived to the lab database so that they can be located by others and posterity. You should also keep a record in your lab notebook of where these samples came from. Instructions for how to use the strain database are located here:

External site Strain Database Instructions

External site Label Templates

Additional information for strains from ATCC

Strains from ATCC typically arrive as freeze-dried samples. After you break the vial, you should resuspend the cells in a ~400 µl of the media suggested by ATCC for growth of your strain. Because these are type strains and we don't want to accidentally select a mutant as our version of the type strain, we archive the following samples:

  • Mixed Population: Immediately add ~100 µl of the resuspension (~1/4 of the total volume) to liquid media. This outgrowth will be the original "mixed population" sample.
  • Clonal Isolates: Streak out from the remainder of the resuspension on a suitable agar plate. Grow as directed, pick 3 colonies to grow in liquid media, and archive as c1, c2, c3. These are the "clonal isolate" samples. The c1 sample will be the one that you use in your experiments and check genetically and phenotypically to be sure it is the correct strain, and not a mutant or contamination!
  • Freeze-Dried: Freeze the remainder of the original resuspension of the freeze-dried culture at –80°C using 10-20% DMSO as cryoprotectant. This is the "original freeze-dried stock".
Added:
>
>
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Revision 52016-03-03 - JeffreyBarrick

 
META TOPICPARENT name="ProtocolList"

Freezing Strains

Supplies

  1. Overnight liquid culture
    Several milliliters of overnight liquid culture grown in a suitable medium for each sample to be frozen.
  2. 80% Glycerol or DMSO solution
    A standard lab solution. Grab your own stock bottle and keep it in your workspace.
  3. Sterile 2 ml cryovials and circular cap inserts
    Found on a shelf above the colony counters in 1.436. Take a bag for yourself and keep it in your workspace, closing it with an alligator clip when not in use.
  4. Cryotag rectangular 1.28" x 0.50" labels
    Found in the bottom drawer of the office supply cabinet below the message board in 1.436.
  5. Clear tape
    Found in dispensers throughout lab or on the office supply cabinet in 1.436. Do NOT use "magic" tape (which is translucent and does not stick as well at –80°C). Use fully clear tape.
  6. Freezer box

Labeling Tubes

  1. Sample naming – Every strain has a three letter designation (usually the initials of someone) and a strain number. When freezing new samples, either append them to your own strain series or obtain the next available numbers from a standard series (e.g. JEB) by looking in the Strain Database.
  2. Write the three letter designation, the strain number, and the date (MM–DD–YY) on a CRYOTAG label for each sample. Also include whatever other distinctive information about the strain that can be fit onto the label (e.g. experiment, population, time).
  3. Stick the label on tube horizontally, and completely cover it with one strip of clear tape for longevity.
  4. Write the strain number on the plastic circular cap insert, so that it will be visible from above when looking down on the tube in a freezer box.

Freezing Samples

You will need to add a cryoprotectant to your sample of cells to be frozen. Generally this is 80% glycerol, though for some experiments DMSO is used instead. The standard amount to add of this cryoprotectant is one-fifth the volume of your cells. This gives a final concentration of 13.3% glycerol or 16.7% DMSO.

If you are using DMSO, wear gloves and avoid contact with your skin!

For most samples, you can follow this procedure:

1 Add 200uL of 80% glycerol to each empty cryovial. Glycerol is extremely viscous. Use the 1 ml pipettor because the tips have a larger aperture. Be careful to pull liquid into the pipette tip slowly and to let excess liquid drip off the outside before you remove the tip from the stock bottle. Use the repeat pipettor if you are freezing >12 samples.

  1. Add 1000uL of each revived strain to the appropriately labeled cryovial using a 1 ml pipettor.
  2. Vortex each cryovial at high speed to be sure that these solutions are uniformly mixed.
  3. Place the tubes in the next positions available in your boxes or the main lab stock boxes. Record the box, rack, and freezer names and numbers.

Updating the Strain Database

It is very important to immediately add information about the samples you have archived to the lab database so that they can be located by others and posterity. You should also keep a record in your lab notebook of where these samples came from. Instructions for how to use the strain database are located here:

External site Strain Database Instructions

External site Label Templates

Added:
>
>

Additional information for strains from ATCC

Strains from ATCC typically arrive as freeze-dried samples. After you break the vial, you should resuspend the cells in a ~400 µl of the media suggested by ATCC for growth of your strain. Because these are type strains and we don't want to accidentally select a mutant as our version of the type strain, we archive the following samples:

  • Mixed Population: Immediately add ~100 µl of the resuspension (~1/4 of the total volume) to liquid media. This outgrowth will be the original "mixed population" sample.
  • Clonal Isolates: Streak out from the remainder of the resuspension on a suitable agar plate. Grow as directed, pick 3 colonies to grow in liquid media, and archive as c1, c2, c3. These are the "clonal isolate" samples. The c1 sample will be the one that you use in your experiments and check genetically and phenotypically to be sure it is the correct strain, and not a mutant or contamination!
  • Freeze-Dried: Freeze the remainder of the original resuspension of the freeze-dried culture at –80°C using 10-20% DMSO as cryoprotectant. This is the "original freeze-dried stock".
 

Revision 42013-09-03 - AlvaroRodriguez

 
META TOPICPARENT name="ProtocolList"

Freezing Strains

Supplies

  1. Overnight liquid culture
    Several milliliters of overnight liquid culture grown in a suitable medium for each sample to be frozen.
  2. 80% Glycerol or DMSO solution
    A standard lab solution. Grab your own stock bottle and keep it in your workspace.
  3. Sterile 2 ml cryovials and circular cap inserts
    Found on a shelf above the colony counters in 1.436. Take a bag for yourself and keep it in your workspace, closing it with an alligator clip when not in use.
  4. Cryotag rectangular 1.28" x 0.50" labels
    Found in the bottom drawer of the office supply cabinet below the message board in 1.436.
  5. Clear tape
    Found in dispensers throughout lab or on the office supply cabinet in 1.436. Do NOT use "magic" tape (which is translucent and does not stick as well at –80°C). Use fully clear tape.
  6. Freezer box

Labeling Tubes

  1. Sample naming – Every strain has a three letter designation (usually the initials of someone) and a strain number. When freezing new samples, either append them to your own strain series or obtain the next available numbers from a standard series (e.g. JEB) by looking in the Strain Database.
  2. Write the three letter designation, the strain number, and the date (MM–DD–YY) on a CRYOTAG label for each sample. Also include whatever other distinctive information about the strain that can be fit onto the label (e.g. experiment, population, time).
  3. Stick the label on tube horizontally, and completely cover it with one strip of clear tape for longevity.
  4. Write the strain number on the plastic circular cap insert, so that it will be visible from above when looking down on the tube in a freezer box.

Freezing Samples

You will need to add a cryoprotectant to your sample of cells to be frozen. Generally this is 80% glycerol, though for some experiments DMSO is used instead. The standard amount to add of this cryoprotectant is one-fifth the volume of your cells. This gives a final concentration of 13.3% glycerol or 16.7% DMSO.

If you are using DMSO, wear gloves and avoid contact with your skin!

For most samples, you can follow this procedure:

1 Add 200uL of 80% glycerol to each empty cryovial. Glycerol is extremely viscous. Use the 1 ml pipettor because the tips have a larger aperture. Be careful to pull liquid into the pipette tip slowly and to let excess liquid drip off the outside before you remove the tip from the stock bottle. Use the repeat pipettor if you are freezing >12 samples.

  1. Add 1000uL of each revived strain to the appropriately labeled cryovial using a 1 ml pipettor.
  2. Vortex each cryovial at high speed to be sure that these solutions are uniformly mixed.
  3. Place the tubes in the next positions available in your boxes or the main lab stock boxes. Record the box, rack, and freezer names and numbers.

Updating the Strain Database

It is very important to immediately add information about the samples you have archived to the lab database so that they can be located by others and posterity. You should also keep a record in your lab notebook of where these samples came from. Instructions for how to use the strain database are located here:

External site Strain Database Instructions

Added:
>
>		 External site Label Templates
 

Revision 32011-06-02 - JeffreyBarrick

 
META TOPICPARENT name="ProtocolList"

Freezing Strains

Changed:
<
<

Items

>
>

Supplies

Deleted:
<
<		1. Obtain a bag 2mL cryovials, currently kept in the shelves above the colony counting machines.
 
Changed:
<
<		2. Keep the bag closed with paperclips and in own workspace while not being used.
>
>
  1. Overnight liquid culture
    Several milliliters of overnight liquid culture grown in a suitable medium for each sample to be frozen.
Added:
>
>
  1. 80% Glycerol or DMSO solution
    A standard lab solution. Grab your own stock bottle and keep it in your workspace.
  2. Sterile 2 ml cryovials and circular cap inserts
    Found on a shelf above the colony counters in 1.436. Take a bag for yourself and keep it in your workspace, closing it with an alligator clip when not in use.
  3. Cryotag rectangular 1.28" x 0.50" labels
    Found in the bottom drawer of the office supply cabinet below the message board in 1.436.
  4. Clear tape
    Found in dispensers throughout lab or on the office supply cabinet in 1.436. Do NOT use "magic" tape (which is translucent and does not stick as well at –80°C). Use fully clear tape.
  5. Freezer box
 
Changed:
<
<		3. Obtain labels from bottom drawer of the cabinet below the message board.
>
>

Labeling Tubes

 
Changed:
<
<		4. Obtain cap circles from _.
>
>
  1. Sample naming – Every strain has a three letter designation (usually the initials of someone) and a strain number. When freezing new samples, either append them to your own strain series or obtain the next available numbers from a standard series (e.g. JEB) by looking in the Strain Database.
Added:
>
>
  1. Write the three letter designation, the strain number, and the date (MM–DD–YY) on a CRYOTAG label for each sample. Also include whatever other distinctive information about the strain that can be fit onto the label (e.g. experiment, population, time).
  2. Stick the label on tube horizontally, and completely cover it with one strip of clear tape for longevity.
  3. Write the strain number on the plastic circular cap insert, so that it will be visible from above when looking down on the tube in a freezer box.
 
Changed:
<
<

Preparing Strains

>
>

Freezing Samples

 
Changed:
<
<		1. Write the three letter initials, the strain number and the time on the label. Also include whatever other distinctive information about the strain that can be fit onto the label.
>
>		You will need to add a cryoprotectant to your sample of cells to be frozen. Generally this is 80% glycerol, though for some experiments DMSO is used instead. The standard amount to add of this cryoprotectant is one-fifth the volume of your cells. This gives a final concentration of 13.3% glycerol or 16.7% DMSO.
 
Changed:
<
<		2. Stick label on tube, and cover it with clear tape for longevity. Also write the strain number on the cap.
>
>		 If you are using DMSO, wear gloves and avoid contact with your skin!
 
Changed:
<
<		3. Steps a and b can be done in either order, however, adding glycerol first is recommended.
>
>		For most samples, you can follow this procedure:
 
Changed:
<
<		 a. Add 200uL of 80% glycerol (found amongst the stock solutions) each cryovial.
>
>		 1 Add 200uL of 80% glycerol to each empty cryovial. Glycerol is extremely viscous. Use the 1 ml pipettor because the tips have a larger aperture. Be careful to pull liquid into the pipette tip slowly and to let excess liquid drip off the outside before you remove the tip from the stock bottle. Use the repeat pipettor if you are freezing >12 samples.
Added:
>
>
  1. Add 1000uL of each revived strain to the appropriately labeled cryovial using a 1 ml pipettor.
  2. Vortex each cryovial at high speed to be sure that these solutions are uniformly mixed.
  3. Place the tubes in the next positions available in your boxes or the main lab stock boxes. Record the box, rack, and freezer names and numbers.
 
Changed:
<
<		 b. Add 1000uL of each revived strain to the appropriately labeled cryovial.
>
>

Updating the Strain Database

 
Changed:
<
<		4. Label the box of cryovials and record the rack and freezer in which it is stored.
>
>		It is very important to immediately add information about the samples you have archived to the lab database so that they can be located by others and posterity. You should also keep a record in your lab notebook of where these samples came from. Instructions for how to use the strain database are located here:
 
Changed:
<
<

Updating the Database

>
>		External site Strain Database Instructions
Deleted:
<
<		 1. Log in to barricklab.org, then log in to lab databases.

2. Click "strains" on the left, then "input." Fill in fields as shown in the chart. Note that the database uses minus signs (–), which it distinguishes from hyphens (-). On a mac, option+hyphen results in a minus sign. Simply put, Ara– is a valid entry, while Ara- is not.

column example description
strain REL Initials of strain designation
number 606 Number of strain designation
freezer Barrick 1 Freezer where sample is located. Choose from list.
rack Barrick 3 Rack where sample is located. Should be in format: [last name] [number]
box Barrick 4 Rack where sample is located. Should be in format: [last name] [number]
container 2 ml glass vial Type of container used to freeze sample. Choose from list.
well   Well number for samples frozen in microplates.
experiment LTEE Sample experiment. Choose from list.
population   Sample population in experiment.)
time 0 Sample time point in experiment.
M/C C Mixed population or Clone sample
clone   Designation of particular clone. Either a number or a letter.
description Ara– ancestor clone used to begin the long-term experiment. Full description of the strain. Include information about what strain it is derived from and whether this sample has been subcultured from different samples.
media DM1000 Media strain was grown in for freezing.
cryoprotectant Glycerol Choose from list.
source REL Stock center or other lab strain is from.
frozen 2002-08-17 Date when sample was frozen.
 

Revision 22011-06-02 - AurkoDasgupta

 
META TOPICPARENT name="ProtocolList"

Freezing Strains

Added:
>
>

Items

1. Obtain a bag 2mL cryovials, currently kept in the shelves above the colony counting machines.

2. Keep the bag closed with paperclips and in own workspace while not being used.

3. Obtain labels from bottom drawer of the cabinet below the message board.

4. Obtain cap circles from _.

Preparing Strains

1. Write the three letter initials, the strain number and the time on the label. Also include whatever other distinctive information about the strain that can be fit onto the label.

2. Stick label on tube, and cover it with clear tape for longevity. Also write the strain number on the cap.

3. Steps a and b can be done in either order, however, adding glycerol first is recommended.

a. Add 200uL of 80% glycerol (found amongst the stock solutions) each cryovial.

b. Add 1000uL of each revived strain to the appropriately labeled cryovial.

4. Label the box of cryovials and record the rack and freezer in which it is stored.

Updating the Database

1. Log in to barricklab.org, then log in to lab databases.

2. Click "strains" on the left, then "input." Fill in fields as shown in the chart. Note that the database uses minus signs (–), which it distinguishes from hyphens (-). On a mac, option+hyphen results in a minus sign. Simply put, Ara– is a valid entry, while Ara- is not.

column example description
strain REL Initials of strain designation
number 606 Number of strain designation
freezer Barrick 1 Freezer where sample is located. Choose from list.
rack Barrick 3 Rack where sample is located. Should be in format: [last name] [number]
box Barrick 4 Rack where sample is located. Should be in format: [last name] [number]
container 2 ml glass vial Type of container used to freeze sample. Choose from list.
well   Well number for samples frozen in microplates.
experiment LTEE Sample experiment. Choose from list.
population   Sample population in experiment.)
time 0 Sample time point in experiment.
M/C C Mixed population or Clone sample
clone   Designation of particular clone. Either a number or a letter.
description Ara– ancestor clone used to begin the long-term experiment. Full description of the strain. Include information about what strain it is derived from and whether this sample has been subcultured from different samples.
media DM1000 Media strain was grown in for freezing.
cryoprotectant Glycerol Choose from list.
source REL Stock center or other lab strain is from.
frozen 2002-08-17 Date when sample was frozen.
 

Revision 12011-06-01 - JeffreyBarrick

 
META TOPICPARENT name="ProtocolList"

Freezing Strains

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