What is the correct pipetting technique?

Depress the plunger to the first stop, immerse the tip into the liquid, and aspirate by releasing the plunger. Remove the pipette from the liquid and depress the plunger to the second stop to dispense the entire contents.

What are the five common pipetting errors?

Here are five common mistakes to avoid when using pipettes: Incorrect calibration. ... Insufficient Tip Attachment. ... An incorrect volume setting. ... Liquid residues and air bubbles: ... Cross-Contamination: ... Aspiration and dispensing errors: ... Technique Inconsistency: ... Tips for Overfilling or Underfilling: More items... Oct 23, 2023

How can I practice pipetting at home?

Practice precisely measuring and mixing small volumes using a Pipette Practice Card and colored dyes . Next, learn the art of loading an electrophoresis gel, a critical tool in the molecular biology lab. Instead of the agarose gel you might encounter in the lab, you'll use a sturdy, reusable silicone practice gel.

How to avoid bubbles when pipetting?

Best Practices to Prevent Air Bubbles Pipette Slowly. ... Use The Correct Immersion Depth. ... Guide To Depth Of Tip Immersion. ... Pre-Wet Pipette Tips. ... Use Reverse Pipetting Techniques If Appropriate. ... ELISA Technique. ... Use Ergonomic Pipettes. ... Take Time to Train Staff. May 16, 2022

Is forward or reverse pipetting more accurate?

Forward pipetting is generally more accurate , especially when transferring small volumes of liquid, while reverse pipetting is generally more efficient, especially when transferring large volumes of liquid.

What not to do when using a pipette?

The following rules apply to all types of pipettes. Never put a pipette in your mouth. Draw the liquid into the pipette using a rubber bulb or pipette pump. Never withdraw a liquid from a near-empty container. ... Never lay a pipette flat on a table or turn upside down with the bulb or pump attached. More items...

How can I make my pipetting more accurate?

Improve Your Pipetting Results with 5 Easy Tips Pre-rinse your new pipette tips before aspirating a sample for delivery. Ensure the tips immersion depth is correct. Ensure the micropipette is upright during pipetting. Apply consistent plunger pressure and speed. Good micropipette. More items... Dec 3, 2019

What is the standard pipetting technique?

For standard pipetting use the forward technique: Press the operating button to the first stop. Dip the tip into the solution to a depth of 1cm, and slowly release the operating button. Withdraw the tip from the liquid, touching it against the edge of the reservoir to remove excess liquid.

What is the first thing you should do when using a pipet?

The first step when using a pipette is setting the pipette to your desired volume . To do this, locate the small window on your pipette that has three numbers in it. If your pipette has a lock/unlock switch, switch it to the unlock position.

Do you push a pipette all the way down?

To do this, you press the pipetting button down onto the first stop. Then you insert the pipette tip into the liquid you want to draw up, and release the pipetting button. Pressing down to the second stop ensures that all the liquid is dispensed .

Guide to Pipetting Techniques | Pipette.com (2024)

Understanding Pipettes

Pipette terms:

Adjustment - altering the pipette so that the dispensed volume is within the specifications.

Air Displacement Pipettes - are meant for general use with aqueous solutions. In air displacement pipettes, a certain volume of air remains between the piston and the liquid.

Aspirate - to draw up the sample.

Blow-out - to empty the tip completely.

Calibration check - checking the difference between the dispensed volume and the selected volume.

Dispense - to deliver the sample.

Positive Displacement Pipettes - are used for high viscosity and volatile liquids. In positive displacement pipettes, the piston is in direct contact with the liquid.

Air Displacement Pipettes

Air Displacement Pipette, used for standard pipetting applications, is highly accurate.

However, conditions such as temperature, atmospheric pressure as well as the specific gravity and viscosity of the solution may have an effect on the performance of air displacement pipettes.

How does an Air Displacement Pipette work?

The piston moves to the appropriate position when the volume is set.
When the operating button is pressed to the first stop, the piston expels thesame volume of air as indicated on the volume setting.
After immersing the tip into the liquid, the operating button is released.This creates a partial vacuum and the specified volume of liquid is aspiratedinto the tip.
When the operating button is pressed to the first stop again, the air dispensesthe liquid. To empty the tip completely the operating button is pressed to the second stop (blow out).

Factors affecting the accuracy of Air Displacement Pipettes:

Temperature
The most important factor in pipetting accuracy is the liquid temperature. The figure below shows the change in volume when the liquid has a different temperature than the pipette and air. If the temperature of the liquid, pipette and air is the same, the accuracy is not significantly affected.

Density
Density is the mass/volume ratio of the liquid. The density varies according to thetemperature and air pressure. Typically, the density of water is 0.996 kg/dm3, for ethanol 0.79 kg/dm3 and for sulfuric acid (H2SO4) 1.85 kg/dm3.

Altitude
The geographic altitude affects the accuracy through the air pressure. The air pressuredecreases at higher altitudes and the conversion factor Z decreases as well. The boiling point of some liquids can also change to quite close to room temperature, increasing the evaporation loss dramatically.

Positive Displacement Pipette

Positive Displacement Pipette, is used for applications like PCR and other DNA amplification techniques. The micro-syringe tips used in positive displacement pipettes are disposable. This helps to avoid sample-to-sample cross-contamination (also known as sample carry-over), and contamination due to the aerosol effect.

How does a positive displacement pipette work?

The piston moves to the appropriate position when the volume is set.
When the operating button is pressed to the stop, the piston descendsto the tip opening.
After the tip is immersed into the liquid, the operating button is released.The plunger is then raised and a partial vacuum is created. This causesthe liquid to enter the tip.
When the operating button is pressed again, the piston descends, expellingthe liquid from the tip.

General guidelines and Pipetting techniques

General guidelines

Check your pipette at the beginning of your working day for dust and dirt onthe outside. If needed, wipe with 70% ethanol.

Set the volume within the range specified for the pipette.

Hold the pipette so the "grippy finger rest" rests on your index finger.

To maximize accuracy, the pipette, tip and liquid should be at the sametemperature.

Check that you are using tips recommended for this pipette. To ensureaccuracy, use only high-quality tips made from contamination-freepolypropylene.

Tips are designed for single use. They should not be cleaned for reuse as theirmetrological characteristics will no longer be reliable.

*Pre-rinsing (1-3 times) the tip with the liquid to be pipetted may improvesaccuracy, especially when using positive displacement tips.

Avoid turning the pipette on its side when there is liquid in the tip. Liquid mightgo to the interior of the pipette and contaminate the pipette.

Avoid contamination to or from fingers by using the tip ejector and gloves.

Forward Pipetting technique

Press the operating button to the first stop.
Dip the tip into the solution to a depth of 1 cm, and slowly release theoperating button. Wait 1-2 seconds and withdraw the tip from the liquid,touching it against the edge of the reservoir to remove excess liquid.
Dispense the liquid into the receiving vessel by gently pressing the operatingbutton to the first stop and then press the operating button to thesecond stop. This action will empty the tip. Remove the tip from the vessel,sliding it up the wall of the vessel.
Release the operating button to the ready position.

Reverse Pipetting technique

The reverse technique is used for pipetting solutions with a high viscosity or a tendencyto foam. Reverse pipetting is only possible with air displacement pipettes

Press the operating button to the second stop.
Dip the tip into the solution to a depth of 1 cm, and slowly release theoperating button. This action will fill the tip with a volume that is larger thanthe set volume. Wait 1-2 seconds and withdraw the tip from the liquid, touching it against the edge of the reservoir to remove excess liquid.
Dispense the liquid into the receiving vessel by pressing the operating buttongently and steadily to the first stop. This volume is equal to the set volume.Hold the button in this position. Some liquid will remain in the tip, and thisshould not be dispensed.
The liquid remaining in the tip can be pipetted back into the original solution ordisposed together with the tip.
Release the operating button to the ready position.

Repetitive Pipetting technique

This technique is intended for repeated pipetting of the same volume. Can only be used with electronic and repeator pipettes.

Press the operating button to the second stop.
Dip the tip into the solution to a depth of 1 cm, and slowly release theoperating button. Withdraw the tip from the liquid, touching it against the edgeof the reservoir to remove excess liquid.
Dispense the liquid into the receiving vessel by gently pressing the operatingbutton to the first stop. Hold the button in this position. Some liquid will remainin the tip, and this should not be dispensed.
Continue pipetting by repeating steps 2 and 3.

Pipetting whole blood

Use forward technique steps 1 and 2 to fill the tip with blood (do not pre-rinse thetip). Wipe the tip carefully with a dry clean cloth.

Dip the tip into the blood and press the operating button to the first stop.Make sure the tip is sufficiently below the surface.
Release the operating button slowly to the ready position. This action will fillthe tip with blood. Do not remove the tip from the solution.
Press the operating button to the first stop and release slowly. Repeat thisprocess until the interior wall of the tip is clear.
Press the operating button to the second stop and completely empty the tip.Remove the tip by sliding it along the wall of the vessel.
Release the operating button to the ready position.

Recommendations for Pipetting different Solutions / Compounds

Solution/Compound	Examples	Pipette	Tip	Technique	Comments
Aqueous solution	Buffers, diluted salt solution	Air Displacement	Standard	Forward
Viscous solution	Protein and nucleic solutions, glycerol, Tween 20/40/60/80	Air DisplacementPos. Displacement	Standard wide orifice Pos. Displacement	Reverse	Pipette slowly to avoid bubble formation.
Volatile compounds	Methanol, Hexane	Air DisplacementPos. Displacement	Filter Pos. Displacement	Forward	Pipette rapidly to avoid evaporation. Carbon filter tips prevent vapors from going into the Pipette.
Nucleotide solutions	Genomic DNA, PCR Products	Air DisplacementPos. Displacement	Filter or wide orifice Pos. Displacement	Forward	For genomic DNA wide orifice should be used to avoid mechanical shearing.
Radioactive compounds	Carbonate, H-thymidine	Air DisplacementPos. Displacement	Filter Pos. Displacement	Forward
Acid / Alkalis	H2SO4, HCI, NaOH	Air Displacement	Filter	Forward
Toxic samples		Pos. Displacement	Pos. Displacement	Forward

Pipetting guidelines for selected compounds

Body Fluids

Whole Blood

Pipette + tip combination: choose an air displacement pipette and a standard or wide orifice tip.
Technique: use the whole blood pipetting technique. Reverse pipetting should be used if high accuracy is needed.
Notice: some blood can remain in the tip and on the outer surface. Wipe the tip against the edge of the vessel to remove excess liquid outside the tip before dispensing.

Serum

Pipette + tip combination: choose an air displacement pipette and a standard or wide orifice tip.
Technique: use the whole blood pipetting technique. Reverse pipetting should be used if high accuracy is needed.
Notice: Residual serum can sometimes be found on the outer surface of the tip. Wipe the tip against the edge of the vessel to remove excess liquid outside the tip before dispensing.

Oily Fluids

Glycerol

Pipette + tip combination: choose an air displacement pipette and a standard or wide orifice tip.
Technique: For high accuracy of performance, use the reverse pipetting technique.
Notice: Oily fluids are difficult to pipette because of formation of air bubbles. Filling must be done very slowly to prevent air bubbles. Wipe the tip against the edge of the vessel to remove excess liquid outside the tip before dispensing. The use of a positive displacement pipette and tip is also useful for pipetting glycerol.

Tween 20, 10% solution

Pipette + tip combination: choose an air displacement pipette and a standard or wide orifice tip.
Technique: use the reverse pipetting technique.
Notice: Tween has a very high viscosity; to make pipetting easier, it should be diluted to a 10% solution. In any case pipetting will not be accurate; some liquid will stay inside the tip. Aspiration and dispensing should be done slowly. The use of a positive displacement pipette and tip is also advisable for pipetting Tween 20.

Bronidox L, 10% (preservative)

Pipette + tip combination: choose an air displacement pipette and a standard or wide orifice tip
Technique: use the reverse pipetting technique.
Notice: Bronidox L is very viscose; the aspiration and dispensing should be done slowly or a positive displacement pipette and tip should be used.

Salt solutions

10 x PBS, 0.1M NaCl, 3M

Pipette + tip combination: choose an air displacement pipette and a standard tip.
Technique: use the forward pipetting technique. Pre-wetting of the tip before aspiration increases accuracy.

Concentrated acids and bases

H2SO4

Pipette + tip combination: choose an air displacement pipette and a filter tip.
Technique: use the forward pipetting technique.

NaOH

Pipette + tip combination: choose an air displacement pipette and a filter tip.
Technique: use the forward pipetting technique.
Notice: some acids or bases vaporize easily (e.g. trifluoroacetic acid). Do the pipetting quite rapidly to minimize vapor formation.

Nucleic acids

For genomic DNA wide orifice should be used to avoid mechanical shearing.

Pipette + tip combination: choose an air displacement pipette and a filter tip or a positive displacement pipette and tip.
Technique: use the forward pipetting technique.
Notice: for genomic DNA wide orifice tips can be used to eliminate mechanical shearing.

Volatile compounds

Pipette + tip combination: choose an air displacement pipette and filter tip or positive displacement pipette and tip.
Technique: use the forward pipetting technique.
Notice: 1.) To get accurate results, calibrate the pipette with the volatile compound you want to pipette. If you use air displacement pipettes, aspirate and dispense the liquid a few times keeping the tip in the liquid. By doing so, the air inside the pipette will be saturated with vapor of the volatile compound. 2.) Pipette rapidly to avoid evaporation when using air displacement pipettes. 3.) It is recommended to use positive displacement pipettes for highly volatile compounds, since the built-in piston tip is in direct contact with the liquid.

Preventing cross-contamination

Pipette-to-sample

A contaminated pipette or contaminated tips can cause contamination of samples.
Prevention:

Use sterilized tips or sterilized filter tips and if possible autoclave the pipette.
Change the tip after pipetting of each sample.

Sample-to-pipette

Samples or aerosols from samples can enter the cone of the pipette.
Prevention:

Keep the pipette vertical when pipetting in order to prevent liquid from runninginto the pipette body.
Release the push-button slowly.
To avoid aerosol contamination, use filter tips or use a positive displacementpipette and tips.
Store the pipette vertically.

Sample-to-sample (carry-over)

The remains of sample A can mix with next sample B inside the tip and may causea false test result.Prevention:

Change the tip after each sample.
If you suspect that your pipette is contaminated, autoclave or clean your pipette.

Tip Selection

One of the most important factors in accurate Pipette measurement is the Tip. The Pipette and the Tip form a System. The best Pipetting results are naturally achieved by those manufactured together to ensure complete compatibility between Pipettors and Pipettor Tip.

Many tips on the market look fine, but when studying them more carefully, it appears that the price really reflects quality. Many of the cheap tips may have flashes, protrusions, and scratches, air bubbles, be bent or contain impurities. All these influence Pipetting results. For example, if the tip is not straight this alone may result in a 10% error in Pipetting accuracy (ISO 8655-2). Moreover, if the tip orifice is not accurately centered, the dispensing of the liquid might be affected significantly. If premium grade pure polypropylene is not used or the mold and processing are not up to the highest standards, part of the liquid stays inside the tip as a droplet, which causes an error in the Pipetting result.

GUIDELINES FOR SELECTING TIPS

All tips should be:

Made to match the Pipettor in use: It is recommended to use tips specified by the manufacturer as well as high quality Unifit tips.
Made of high quality pure virgin polypropylene
Free from dust or particles
Uniform in size and shape
Accurately centered for tip orifice
Free from metals, like cadmium
Securely sealed: There should be good tip cone match for a perfect seal and tip eject
Free from blemishes, flashing or any protrusions
Highly resistant to chemicals
Highly stable thermally
Autoclavable or presterilised for use in sterile applications
Traceable: Lot numbers and mold cavity identification markings in each tip

Calibrating your Pipettes

Calibration of Pipettes

Device requirements and test conditions

Balance:

The scale graduation value of the balance should be chosen according to the selected pipette volume.

Volume range	Readable graduation
Under 50 vl	0.001 mg
Above 50 vl	0.01 mg

Note: check the calibration of your balance regularly using known weights.

Test liquid:

Water, distilled or de-ionized, "Grade 3", conforming to ISO 3696. The test water isheld in the calibration room for at least 2 hours before calibration to reach equilibriumwith the test room conditions.

Test room:

Tests are performed in a draught-free room at a constant (+/- 0.5C) temperature of 20C to 25C. Relative humidity is recommended to be above 45%. Especially with volumes under 50 vl, the air humidity should be as high as possible to reduce the evaporation loss effect.

- The pipette, the water and the air in the test room should be at the sametemperature.

- A new tip should be pre-wetted 1 to 3 times to improve the accuracy.

- Always pipette water from a reservoir, do not take it back from the balance.

- Check the calibration regularly, depending on the frequency of use and on theapplication, but at least once a year. If used daily, a three-month interval isrecommended.

Procedures to check calibration:

General Pipette Calibration Procedure

Incoming Inspection procedure

Upon receipt, each Pipette carefully unpacked and inspected for any signs of visible damage.
- Any visible damage found is reported back to customer immediately. Customer will be advised if the damage is Repairable and what additional cost will be charged. Customer will issue a new Work Order to cover the cost of Repair.
Afterwards each Pipette is scanned for radiation contamination.
- Any radiation contamination discovered is reported back to customer immediately, and Pipette is Rejected.
All customer Pipettes are counted and compared to quantity reported on supplied Work Order.
- Any quantity discrepancies are reported back to the customer immediately. Customer will have opportunity to locate any missing quantities, or Work Order will need to be revised and revision signed by Customer.
Each Work Order will be placed in a separate in-house storage box until scheduled for Calibration.
Separate Job ID numbers are assigned for every Work Order.
Customer information is checked for any discrepancies from that on file and will be corrected, if needed. If this is a New Customer, a Customer information file will be started.
All Pipettes are entered in Cal Lab database under assigned Job ID number with ID number assigned to each instrument.

Pre-calibration procedure

As Found� data obtained and recorded prior to Calibration and any Pipette adjustments are also recorded.
Each Pipette will be tested at lowest and highest range points as specified by manufacture. Ten tests performed at each point.
As part of Preventive Maintenance, each Pipette disassembled according to manufacturer�s diagrams and cleaned thoroughly with the appropriate chemical solutions.
All parts are carefully inspected, piston is polished in most cases, piston seal and o-ring are replaced as well as all defective and malfunctioning parts. [see 12-Point Inspection diagram]
Upon completion each Pipette is reassembled according to the manufacturer�s diagram and procedures. Pipette is again visually checked for proper functionality.
Calibration procedure
At the start of Calibration, each Pipette pre-checked 3 times before any adjustments are done. If Pipette fails, appropriate Calibration adjustments are performed. After corrections, each instrument will be Calibrated at the lowest and highest range points with 10 tests at each test point.
Calibration Data will be recorded and reported on a Calibration Report.
Calibration reports are issued for each Pipette as well as Calibration Summary for the whole job. Appropriate technicians sign reports.
Calibration Label created and attached to each Pipette.
All Pipettes crosschecked back to customer supplied paperwork as well as in-lab created documentation.
Randomly selected Pipettes are checked for overall performance by QC Supervisor.
- If any error is detected, the entire Job is sent back for recheck.
QC Supervisor approves Job, and Pipette is carefully packaged and delivered to customer with all Calibration Documentation enclosed.

Calibration

The pipette is held in the calibration room for at least 2 hours before calibrationto reach equilibrium with the test room conditions.
The pipette is checked at the maximum volume (nominal volume) and at theminimum volume or 10% of the maximum volume, whichever is higher.
A series of ten pipettings is performed with both volumes.
Calculate the accuracy and precision using the Formulas section below. If the calculated results are within the limits given in the Instructions-for-use booklet, the pipette calibration is correct. If not, the pipette has to be adjusted with the lower volume and checked again.

Sources of pipette error:

Volatile liquids evaporate. Use in saturated air.
High density liquids sink. Change technique.
Viscous liquids stick to tip. Change technique.
Hydrophilic tips will retain liquid. Pre-wet tip.
Immersed tips carry over liquid. Immerse 2-3mm.
Angled pipettes take up more liquid. Keep vertical.
Surface tension reduces accuracy. Change technique.
Hot and cold liquids. Pipette liquids at room temp.
The human factor. Practice and observe technique.

Procedures to adjust the pipette:

Manual pipettes

The adjustment is done at the lower volume.
Place the service tool that comes with the pipette into the openings of the calibration nut at the top of the handle.
Turn the service tool clockwise to increase the volume or counter clockwise todecrease the volume.
After the adjustment, check the calibration as described above.

Electronic pipettes

Please follow specific manufacturers� instructions due to substantial variations in calibration procedure.

Formulas for calculating results

Conversion of mass to volume

V = (w + e) x Z

V = volume (vl)

w = weight (mg)

e = evaporation loss (mg)

Z = conversion factor for mg/vl conversion

Note: evaporation loss can be significant with low volumes. To determine mass loss, dispense water into the weighing vessel, note the reading and begin timing with astopwatch. Check how much the reading decreases during the 5 seconds. Comparethis to the pipetting time. Typically, the pipetting time might be 5 seconds and the mass loss up to 2 mg. If an evaporation trap or lid on the vessel is used, an evaporation correction is unnecessary.

The conversion factor Z is for calculating the density of water suspended in air atthe test temperature and pressure. See the conversion Table 1 on page 15.

Accuracy (systematic error)

Accuracy is the difference between the dispensed volume and the selected volume of a pipette.

Accuracy is expressed on the calibration certificate as a relative value:

Precision (random error)
Precision refers to the repeatability of the pipettings. It is expressed as standarddeviation (s) or coefficient of variation (cv). In addition to the features of the pipette,laboratory practice and user experience are the main factors affecting precision.

Error according to DIN 12650 (F-value)

The DIN standard does not give individual limits for accuracy and precision, butuses a combined error limit: the F-value.

F = | A | + 2 x s

The relative F-value is calculated:

F% = | A% | + 2 x cv

Table 2 shows the error limit according to the DIN 12650 standard for single-channelair displacement pipettes. For multichannel pipettes, these limits are doubled. With variable volume pipettes, the nominal volume is the maximum volume. The absolute vl limit of the nominal volume applies to every selected volume throughout the volume range.

For example, for a 20 - 200 vl pipette, the error limit is 2.0 vl for every selected volume. If the nominal volume of the pipette is between those in the table, the relative error limit F% of the nearest volume is used. If the nominal volume is exactly between the two volumes in Table 2, the relative error limit F% of the lower volume is used.

Table:
DIN 12650 error limits for single channel air displacement pipettes

Best Practices

Ensuring optimum performance

Error-free pipetting requires both precision and accuracy. A number of factors caneffect these specifications, which are the main quantitative parameters for evaluatingpipette performance.

What are accuracy and precision?

For example when the set volume is 20 vl:

Accurate, but not precise: The mean volume is the correct (set) volume, butseparate pipettings differ from the set volume.

Precise, but not accurate: There is no variation between the separate pipettings,but the mean volume differs from the set volume.

Accurate and precise: The mean volume is the set volume and there is no variation between different pipettings.

1. Pipette vertical, tip immersed about 1 cm into the liquid.

2. Pipette vertical, tip immersed about 3 cm into the liquid.

3. Pipette at a 30 � 40 degree angle; tip immersed about 3-4 cm into the liquid.

Autoclaving (Sterilization)

Please, follow these instructions carefully in order to avoid damage to tips and pipettes.

Autoclave tips at 121�C (248'F) for 20 minutes. Immediately after autoclaving,the tips are moist. Allow moisture to evaporate before using the tips, preferablyovernight.
Some digital model Pipettes can be autoclaved in one piece at 121'C (248'F)for 20 minutes. The tip cone modules of the single-channel models can also be autoclaved.
After autoclaving, the pipette must be cooled at room temperature for at leasttwo hours before use.
Check the calibration of the pipette after every autoclave treatment.

Note: Autoclaving has a limited spectrum of action and will not destroy RNA for example. It is also important to note that certain parts of a pipette - for instance the piston and the handle cannot be autoclaved without altering accuracy and precision

General guidelines for decontaminating Pipettes when Working with Different Liquids

General liquid handling questions

Question:
What is the difference between air displacement and positive displacement pipettes?

Answer:Both types of pipettes have a piston that moves in a cylinder, or capillary. In air displacement pipettes, a specified volume of air remains between the piston and theliquid. In positive displacement pipettes, the piston is in direct contact with the liquid.This keeps air from entering the tip, preventing contamination effectively. Airdisplacement pipettes are meant for general use with aqueous solutions. Positivedisplacement pipettes are used for high viscosity and volatile liquids.

Question:
How can I pipette viscous liquids?

Answer:
You can do so using an air displacement pipette with standard or wide orifice tip(reverse pipetting, slowly). An alternative to this is to use a positive displacementsystem.

Question:
How can I prevent liquid dropping out of the tip when pipetting volatile compounds?

Answer:
If you use air displacement pipettes, aspirate and dispense the liquid a few timeskeeping the tip in the liquid. By doing so, the air inside the pipette will be saturatedwith vapor of the volatile compound. It is recommend using positive displacementpipettes for highly volatile compounds, since the built-in piston tip is in direct contact with the liquid.

Question:
How accurately can I pipette warm or cold liquids.

Answer:
The pipettes are calibrated by weighing distilled or de-ionized water of 20 - 25C.With warm liquids, you will get a smaller mass with a certain volume, with cold liquids,you will get a higher mass.