|
|
| (2 intermediate revisions not shown) |
| Line 10: |
Line 10: |
| | inoculating loop, culture tubes and flasks, 37°C shaking incubator, and centrifuge | | inoculating loop, culture tubes and flasks, 37°C shaking incubator, and centrifuge |
| | with rotor and tubes or bottles for harvesting cells) | | with rotor and tubes or bottles for harvesting cells) |
| | + | |
| | ■ QIArack or equivalent holder (see “Setup of QIAGEN-tips”, page 13) | | ■ QIArack or equivalent holder (see “Setup of QIAGEN-tips”, page 13) |
| | + | |
| | ■ Ice | | ■ Ice |
| | + | |
| | ■ Isopropanol | | ■ Isopropanol |
| | + | |
| | ■ 70% ethanol | | ■ 70% ethanol |
| | + | |
| | ■ Plasmid resuspension buffer (e.g., TE buffer, pH 8.0, or Tris·Cl, pH 8.5) | | ■ Plasmid resuspension buffer (e.g., TE buffer, pH 8.0, or Tris·Cl, pH 8.5) |
| - | For QIAGEN Plasmid Mini Kit protocol: | + | |
| | + | ''For QIAGEN Plasmid Mini Kit protocol:'' |
| | + | |
| | ■ Microcentrifuge | | ■ Microcentrifuge |
| | + | |
| | ■ 1.5 ml or 2 ml microcentrifuge tubes | | ■ 1.5 ml or 2 ml microcentrifuge tubes |
| - | For QIAGEN Plasmid Midi, Maxi, Mega, and Giga Kit protocols: | + | |
| | + | ''For QIAGEN Plasmid Midi, Maxi, Mega, and Giga Kit protocols:'' |
| | + | |
| | ■ Centrifugation tubes or vessels with suitable capacity for the volumes specified in the | | ■ Centrifugation tubes or vessels with suitable capacity for the volumes specified in the |
| | appropriate protocol. | | appropriate protocol. |
| | + | |
| | ■ Refrigerated centrifuge capable of ≥20,000 x g with rotor for the appropriate | | ■ Refrigerated centrifuge capable of ≥20,000 x g with rotor for the appropriate |
| | centrifuge tubes or bottles | | centrifuge tubes or bottles |
| Line 26: |
Line 37: |
| | [[Protocol: Plasmid or Cosmid DNA Purification Using QIAGEN Plasmid Mini Kit]] | | [[Protocol: Plasmid or Cosmid DNA Purification Using QIAGEN Plasmid Mini Kit]] |
| | | | |
| - | This protocol is designed for preparation of up to 20 μg of high-copy plasmid or cosmid
| + | [[Protocol: Plasmid or Cosmid DNA Purification Using QIAGEN Plasmid Midi and Maxi Kits]] |
| - | DNA using the QIAGEN Plasmid Mini Kit. For additional protocols, such as for cosmid,
| + | |
| - | low-copy-number plasmid, BACs, PACs, P1s, and double-stranded M13 replicative form
| + | |
| - | purification, see the recommendations at www.qiagen.com/goto/plasmidinfo .
| + | |
| - | | + | |
| - | ''Important notes before starting''
| + | |
| - | | + | |
| - | ■ New users are advised to familiarize themselves with the detailed protocol provided
| + | |
| - | in this handbook. In addition, extensive background information is provided on our
| + | |
| - | plasmid resource page www.qiagen.com/goto/plasmidinfo .
| + | |
| - | ■ Optional: Remove samples at the steps indicated with the symbol ☞ in order to
| + | |
| - | monitor the procedure on an analytical gel (see page 41)
| + | |
| - | Things to do before starting
| + | |
| - | ■ Add the provided RNase A solution to Buffer P1 before use. Use one vial of RNase
| + | |
| - | A (centrifuge briefly before use) per bottle of Buffer P1, to give a final concentration
| + | |
| - | of 100 μg/ml.
| + | |
| - | ■ Check Buffer P2 for SDS precipitation due to low storage temperatures. If necessary,
| + | |
| - | dissolve the SDS by warming to 37°C.
| + | |
| - | ■ Pre-chill Buffer P3 at 4°C.
| + | |
| - | ■ Optional: Add the provided LyseBlue reagent to Buffer P1 and mix before use. Use
| + | |
| - | one vial LyseBlue (centrifuge briefly before use) per bottle of Buffer P1 to achieve a
| + | |
| - | 1:1000 dilution. LyseBlue provides visual identification of optimum buffer mixing
| + | |
| - | thereby preventing the common handling errors that lead to inefficient cell lysis and
| + | |
| - | incomplete precipitation of SDS, genomic DNA, and cell debris.
| + | |
| - | | + | |
| - | ''Procedure''
| + | |
| - | | + | |
| - | 1. Pick a single colony from a freshly streaked selective plate and inoculate a starter
| + | |
| - | culture of 2–5 ml LB medium containing the appropriate selective antibiotic. Incubate
| + | |
| - | for approximately 8 h at 37°C with vigorous shaking (approx. 300 rpm).
| + | |
| - | Use a tube or flask with a volume of at least 4 times the volume of the culture.
| + | |
| - | 2. Dilute the starter culture 1/500 to 1/1000 into 3 ml selective LB medium. Grow at
| + | |
| - | 37°C for 12–16 h with vigorous shaking (approx. 300 rpm).
| + | |
| - | Use a flask or vessel with a volume of at least 4 times the volume of the culture. The
| + | |
| - | culture should reach a cell density of approximately 3–4 x 109 cells per milliliter,
| + | |
| - | which typically corresponds to a pellet wet weight of approximately 3 g/liter
| + | |
| - | medium.
| + | |
| - | 3. Harvest the bacterial cells by centrifugation at 6000 x g for 15 min at 4°C.
| + | |
| - | ƒ If you wish to stop the protocol and continue later, freeze the cell pellets at –20°C.
| + | |
| - | 4. Resuspend the bacterial pellet in 0.3 ml of Buffer P1.
| + | |
| - | Ensure that RNase A has been added to Buffer P1.
| + | |
| - | If LyseBlue reagent has been added to Buffer P1, vigorously shake the buffer bottle
| + | |
| - | before use to ensure LyseBlue particles are completely resuspended. The bacteria
| + | |
| - | should be resuspended completely by vortexing or pipetting up and down until no
| + | |
| - | cell clumps remain.
| + | |
| - | 5. Add 0.3 ml of Buffer P2, mix thoroughly by vigorously inverting the sealed tube
| + | |
| - | 4–6 times, and incubate at room temperature (15–25°C) for 5 min.
| + | |
| - | Do not vortex, as this will result in shearing of genomic DNA. The lysate should
| + | |
| - | appear viscous. Do not allow the lysis reaction to proceed for more than 5 min. After
| + | |
| - | use, the bottle containing Buffer P2 should be closed immediately to avoid
| + | |
| - | acidification from CO2 in the air.
| + | |
| - | If LyseBlue has been added to Buffer P1 the cell suspension will turn blue after
| + | |
| - | addition of Buffer P2. Mixing should result in a homogeneously colored suspension.
| + | |
| - | If the suspension contains localized colorless regions or if brownish cell clumps are
| + | |
| - | still visible, continue mixing the solution until a homogeneously colored suspension
| + | |
| - | is achieved.
| + | |
| - | 6. Add 0.3 ml of chilled Buffer P3, mix immediately and thoroughly by vigorously
| + | |
| - | inverting 4–6 times, and incubate on ice for 5 min.
| + | |
| - | Precipitation is enhanced by using chilled Buffer P3 and incubating on ice. After
| + | |
| - | addition of Buffer P3, a fluffy white material forms and the lysate becomes less
| + | |
| - | viscous. The precipitated material contains genomic DNA, proteins, cell debris, and
| + | |
| - | KDS. The lysate should be mixed thoroughly to ensure even potassium dodecyl
| + | |
| - | sulphate precipitation. If the mixture still appears viscous, more mixing is required to
| + | |
| - | completely neutralize the solution.
| + | |
| - | If LyseBlue reagent has been used, the suspension should be mixed until all trace of
| + | |
| - | blue has gone and the suspension is colorless. A homogeneous colorless suspension
| + | |
| - | indicates that the SDS has been effectively precipitated.
| + | |
| - | 7. Centrifuge at maximum speed in a microcentrifuge for 10 min. Remove supernatant
| + | |
| - | containing plasmid DNA promptly.
| + | |
| - | Before loading the centrifuge, the sample should be mixed again. Centrifugation
| + | |
| - | should be performed at maximum speed in 1.5 ml or 2 ml microcentrifuge tubes
| + | |
| - | (e.g., 10,000–13,000 rpm in a microcentrifuge). Maximum speed corresponds to
| + | |
| - | 14,000–18,000 x g for most microcentrifuges. After centrifugation, the supernatant
| + | |
| - | should be clear. If the supernatant is not clear, a second, shorter centrifugation should
| + | |
| - | be carried out to avoid applying any suspended or particulate material to the column.
| + | |
| - | Suspended material (which causes the sample to appear turbid) will clog the column
| + | |
| - | and reduce or eliminate flow.
| + | |
| - | ☞ Remove a 50 μl sample from the cleared lysate and save it for an analytical gel
| + | |
| - | (sample 1).
| + | |
| - | 8. Equilibrate a QIAGEN-tip 20 by applying 1 ml Buffer QBT, and allow the column to
| + | |
| - | empty by gravity flow.
| + | |
| - | Place QIAGEN-tips into a QIArack over the waste tray or use the tip holders provided
| + | |
| - | with each kit (see “Setup of QIAGEN-tips” page 13). Flow of buffer will begin
| + | |
| - | automatically by reduction in surface tension due to the presence of detergent in the
| + | |
| - | equilibration buffer. Allow the QIAGEN-tip to drain completely. QIAGEN-tips can
| + | |
| - | be left unattended, since the flow of buffer will stop when the meniscus reaches the
| + | |
| - | upper frit in the column.
| + | |
| - | 9. Apply the supernatant from step 7 to the QIAGEN-tip 20 and allow it to enter the
| + | |
| - | resin by gravity flow.
| + | |
| - | The supernatant should be loaded onto the QIAGEN-tip promptly. If it is left too long
| + | |
| - | and becomes cloudy due to further precipitation of protein, it must be centrifuged
| + | |
| - | again before loading to prevent clogging of the QIAGEN-tip.
| + | |
| - | ☞ Remove a 50 μl sample of the flow-through and save for an analytical gel
| + | |
| - | (sample 2).
| + | |
| - | 10. Wash the QIAGEN-tip 20 with 2 x 2 ml Buffer QC.
| + | |
| - | Allow Buffer QC to move through the QIAGEN-tip by gravity flow.
| + | |
| - | ☞ Remove a 220 μl sample of the combined wash fractions and save for an
| + | |
| - | analytical gel (sample 3).
| + | |
| - | 11. Elute DNA with 0.8 ml Buffer QF.
| + | |
| - | Collect the eluate in a 1.5 ml or 2 ml microcentrifuge tubes (not supplied).
| + | |
| - | Note: For constructs larger than 45–50 kb, prewarming the elution buffer to 65°C
| + | |
| - | may help to increase yield.
| + | |
| - | ☞ Remove a 45 μl sample of the eluate and save for an analytical gel (sample 4).
| + | |
| - | 12. Precipitate DNA by adding 0.7 volumes (0.56 ml per 0.8 ml of elution volume) of
| + | |
| - | room-temperature isopropanol to the eluted DNA. Mix and centrifuge immediately
| + | |
| - | at ≥10,000 rpm for 30 min in a microcentrifuge. Carefully decant the supernatant.
| + | |
| - | All solutions should be at room temperature in order to minimize salt precipitation.
| + | |
| - | Isopropanol pellets have a glassy appearance and may be more difficult to see than
| + | |
| - | the fluffy, salt-containing pellets that result from ethanol precipitation. Marking the
| + | |
| - | outside of the tube before centrifugation allows the pellet to be easily located.
| + | |
| - | Isopropanol pellets are also more loosely attached to the side of the tube, and care
| + | |
| - | should be taken when removing the supernatant.
| + | |
| - | 13. Wash DNA pellet with 1 ml of 70% ethanol and centrifuge at 10,000 rpm for 10 min.
| + | |
| - | Carefully decant the supernatant without disturbing the pellet.
| + | |
| - | The 70% ethanol removes precipitated salt and replaces isopropanol with the more
| + | |
| - | volatile ethanol, making the DNA easier to redissolve.
| + | |
| - | 14. Air-dry the pellet for 5–10 min, and redissolve the DNA in a suitable volume of buffer
| + | |
| - | (e.g., TE buffer, pH 8.0, or 10mM Tris·Cl, pH 8.5)
| + | |
| - | Redissolve the DNA pellet by rinsing the walls to recover all the DNA. Pipetting the
| + | |
| - | DNA up and down to promote resuspension may cause shearing and should be
| + | |
| - | avoided. Overdrying the pellet will make the DNA difficult to redissolve. DNA
| + | |
| - | dissolves best under slightly alkaline conditions; it does not easily dissolve in acidic
| + | |
| - | buffers.
| + | |
| - | Determination of yield
| + | |
| - | To determine the yield, DNA concentration should be determined by both UV
| + | |
| - | spectrophotometry at 260 nm and quantitative analysis on an agarose gel. For reliable
| + | |
| - | spectrophotometric DNA quantification, A260 readings should lie between 0.1 and 1.0.
| + | |
| - | Agarose gel analysis
| + | |
| - | We recommend removing and saving aliquots during the purification procedure
| + | |
| - | (samples 1–4). If the plasmid DNA is of low yield or quality, the samples can be
| + | |
| - | analyzed by agarose gel electrophoresis to determine at what stage of the purification
| + | |
| - | procedure the problem occurred
| + | |
| - | | + | |
| - | | + | |
| - | | + | |
| - | | + | |
| - | [[Protocol: Plasmid or Cosmid DNA Purification Using | + | |
| - | QIAGEN Plasmid Midi and Maxi Kits]] | + | |
| - | | + | |
| - | ''Procedure''
| + | |
| - | | + | |
| - | 1. Pick a single colony from a freshly streaked selective plate and inoculate a starter
| + | |
| - | culture of 2–5 ml LB medium containing the appropriate selective antibiotic. Incubate
| + | |
| - | for approx. 8 h at 37°C with vigorous shaking (approx. 300 rpm).
| + | |
| - | Use a tube or flask with a volume of at least 4 times the volume of the culture.
| + | |
| - | 2. Dilute the starter culture 1/500 to 1/1000 into selective LB medium. For high-copy
| + | |
| - | plasmids, inoculate ▲ 25 ml or ● 100 ml medium with ▲ 25–50 μl or
| + | |
| - | ● 100–200 μl of starter culture. For low-copy plasmids, inoculate ▲ 100 ml or
| + | |
| - | ● 500 ml medium with ▲ 100–200 μl or ● 250–500 μl of starter culture. Grow at
| + | |
| - | 37°C for 12–16 h with vigorous shaking (approx. 300 rpm).
| + | |
| - | Use a flask or vessel with a volume of at least 4 times the volume of the culture. The
| + | |
| - | culture should reach a cell density of approximately 3–4 x 109 cells per milliliter,
| + | |
| - | which typically corresponds to a pellet wet weight of approximately 3 g/liter
| + | |
| - | medium.
| + | |
| - | 3. Harvest the bacterial cells by centrifugation at 6000 x g for 15 min at 4°C.
| + | |
| - | ƒ If you wish to stop the protocol and continue later, freeze the cell pellets at –20°C.
| + | |
| - | 4. Resuspend the bacterial pellet in ▲ 4 ml or ● 10 ml Buffer P1.
| + | |
| - | For efficient lysis it is important to use a vessel that is large enough to allow complete
| + | |
| - | mixing of the lysis buffers. Ensure that RNase A has been added to Buffer P1.
| + | |
| - | If LyseBlue reagent has been added to Buffer P1, vigorously shake the buffer bottle
| + | |
| - | before use to ensure LyseBlue particles are completely resuspended. The bacteria
| + | |
| - | should be resuspended completely by vortexing or pipetting up and down until no
| + | |
| - | cell clumps remain.
| + | |
| - | 5. Add ▲ 4 ml or ● 10 ml Buffer P2, mix thoroughly by vigorously inverting the sealed
| + | |
| - | tube 4–6 times, and incubate at room temperature (15–25°C) for 5 min.
| + | |
| - | Do not vortex, as this will result in shearing of genomic DNA. The lysate should
| + | |
| - | appear viscous. Do not allow the lysis reaction to proceed for more than 5 min. After
| + | |
| - | use, the bottle containing Buffer P2 should be closed immediately to avoid
| + | |
| - | acidification from CO2 in the air.
| + | |
| - | If LyseBlue has been added to Buffer P1 the cell suspension will turn blue after
| + | |
| - | addition of Buffer P2. Mixing should result in a homogeneously colored suspension.
| + | |
| - | If the suspension contains localized colorless regions or if brownish cell clumps are
| + | |
| - | still visible, continue mixing the solution until a homogeneously colored suspension
| + | |
| - | is achieved.
| + | |
| - | 6. Add ▲ 4 ml or ● 10 ml of chilled Buffer P3, mix immediately and thoroughly by
| + | |
| - | vigorously inverting 4–6 times, and incubate on ice for ▲ 15 min or ● 20 min.
| + | |
| - | Precipitation is enhanced by using chilled Buffer P3 and incubating on ice. After
| + | |
| - | addition of Buffer P3, a fluffy white material forms and the lysate becomes less
| + | |
| - | viscous. The precipitated material contains genomic DNA, proteins, cell debris, and
| + | |
| - | KDS. The lysate should be mixed thoroughly to ensure even potassium dodecyl sulfate
| + | |
| - | precipitation. If the mixture still appears viscous, more mixing is required to
| + | |
| - | completely neutralize the solution.
| + | |
| - | If LyseBlue reagent has been used, the suspension should be mixed until all trace of
| + | |
| - | blue has gone and the suspension is colorless. A homogeneous colorless suspension
| + | |
| - | indicates that the SDS has been effectively precipitated.
| + | |
| - | 7. Centrifuge at ≥20,000 x g for 30 min at 4°C. Remove supernatant containing plasmid
| + | |
| - | DNA promptly.
| + | |
| - | Before loading the centrifuge, the sample should be mixed again. Centrifugation
| + | |
| - | should be performed in non-glass tubes (e.g., polypropylene). After centrifugation
| + | |
| - | the supernatant should be clear.
| + | |
| - | Note: Instead of centrifugation steps 7 and 8, the lysate can be efficiently cleared by
| + | |
| - | filtration using a QIAfilter Kits or Cartridges (see www.qiagen.com/products/
| + | |
| - | plasmid/LargeScaleKits).
| + | |
| - | 8. Centrifuge the supernatant again at ≥20,000 x g for 15 min at 4°C. Remove
| + | |
| - | supernatant containing plasmid DNA promptly.
| + | |
| - | This second centrifugation step should be carried out to avoid applying suspended
| + | |
| - | or particulate material to the QIAGEN-tip. Suspended material (causing the sample
| + | |
| - | to appear turbid) can clog the QIAGEN-tip and reduce or eliminate gravity flow.
| + | |
| - | ☞ Remove a ▲ 240 μl or ● 120 μl sample from the cleared lysate supernatant and
| + | |
| - | save for an analytical gel (sample 1) in order to determine whether growth and
| + | |
| - | lysis conditions were optimal.
| + | |
| - | 9. Equilibrate a ▲ QIAGEN-tip 100 or ● QIAGEN-tip 500 by applying ▲ 4 ml or
| + | |
| - | ● 10 ml Buffer QBT, and allow the column to empty by gravity flow.
| + | |
| - | Flow of buffer will begin automatically by reduction in surface tension due to the
| + | |
| - | presence of detergent in the equilibration buffer. Allow the QIAGEN-tip to drain
| + | |
| - | completely. QIAGEN-tips can be left unattended, since the flow of buffer will stop
| + | |
| - | when the meniscus reaches the upper frit in the column.
| + | |
| - | 10. Apply the supernatant from step 8 to the QIAGEN-tip and allow it to enter the resin
| + | |
| - | by gravity flow.
| + | |
| - | The supernatant should be loaded onto the QIAGEN-tip promptly. If it is left too long
| + | |
| - | and becomes cloudy due to further precipitation of protein, it must be centrifuged
| + | |
| - | again or filtered before loading to prevent clogging of the QIAGEN-tip.
| + | |
| - | ☞ Remove a ▲ 240 μl or ● 120 μl sample from the flow-through and save for an
| + | |
| - | analytical gel (sample 2) in order to determine the efficiency of DNA binding to
| + | |
| - | the QIAGEN Resin.
| + | |
| - | 11. Wash the QIAGEN-tip with ▲ 2 x 10 ml or ● 2 x 30 ml Buffer QC.
| + | |
| - | Allow Buffer QC to move through the QIAGEN-tip by gravity flow. The first wash is
| + | |
| - | sufficient to remove all contaminants in the majority of plasmid DNA preparations.
| + | |
| - | The second wash is especially necessary when large culture volumes or bacterial
| + | |
| - | strains producing large amounts of carbohydrates are used.
| + | |
| - | ☞ Remove a ▲ 400 μl or ● 240 μl sample from the combined wash fractions and
| + | |
| - | save for an analytical gel (sample 3).
| + | |
| - | 12. Elute DNA with ▲ 5 ml or ● 15 ml Buffer QF.
| + | |
| - | Collect the eluate in a 15 ml or 50 ml tube (not supplied). Use of polycarbonate
| + | |
| - | centrifuge tubes is not recommended as polycarbonate is not resistant to the alcohol
| + | |
| - | used in subsequent steps.
| + | |
| - | Note: For constructs larger than 45–50 kb, prewarming the elution buffer to 65°C
| + | |
| - | may help to increase yield.
| + | |
| - | ☞ Remove a ▲ 100 μl or ● 60 μl sample of the eluate and save for an analytical
| + | |
| - | gel (sample 4).
| + | |
| - | ƒ If you wish to stop the protocol and continue later, store the eluate at 4°C. Storage
| + | |
| - | periods longer than overnight are not recommended.
| + | |
| - | 13. Precipitate DNA by adding ▲ 3.5 ml or ● 10.5 ml (0.7 volumes) room-temperature
| + | |
| - | isopropanol to the eluted DNA. Mix and centrifuge immediately at ≥15,000 x g for
| + | |
| - | 30 min at 4°C. Carefully decant the supernatant.
| + | |
| - | All solutions should be at room temperature in order to minimize salt precipitation,
| + | |
| - | although centrifugation is carried out at 4°C to prevent overheating of the sample.
| + | |
| - | Alternatively, disposable conical bottom centrifuge tubes can be used for
| + | |
| - | centrifugation at 5000 x g for 60 min at 4°C. Isopropanol pellets have a glassy
| + | |
| - | appearance and may be more difficult to see than the fluffy, salt-containing pellets
| + | |
| - | that result from ethanol precipitation. Marking the outside of the tube before
| + | |
| - | centrifugation allows the pellet to be more easily located. Isopropanol pellets are also
| + | |
| - | more loosely attached to the side of the tube, and care should be taken when
| + | |
| - | removing the supernatant.
| + | |
| - | 14. Wash DNA pellet with ▲ 2 ml or ● 5 ml of room-temperature 70% ethanol, and
| + | |
| - | centrifuge at ≥15,000 x g for 10 min. Carefully decant the supernatant without
| + | |
| - | disturbing the pellet.
| + | |
| - | Alternatively, disposable conical-bottom centrifuge tubes can be used for
| + | |
| - | centrifugation at 5000 x g for 60 min at 4°C. The 70% ethanol removes precipitated
| + | |
| - | salt and replaces isopropanol with the more volatile ethanol, making the DNA easier
| + | |
| - | to redissolve.
| + | |
| - | 15. Air-dry the pellet for 5–10 min, and redissolve the DNA in a suitable volume of buffer
| + | |
| - | (e.g., TE buffer, pH 8.0, or 10 mM Tris·Cl, pH 8.5).
| + | |
| - | Redissolve the DNA pellet by rinsing the walls to recover all the DNA, especially if
| + | |
| - | glass tubes have been used. Pipetting the DNA up and down to promote
| + | |
| - | resuspension may cause shearing and should be avoided. Overdrying the pellet will
| + | |
| - | make the DNA difficult to redissolve. DNA dissolves best under slightly alkaline
| + | |
| - | conditions; it does not easily dissolve in acidic buffers.
| + | |
| - | Determination of yield
| + | |
| - | To determine the yield, DNA concentration should be determined by both UV
| + | |
| - | spectrophotometry at 260 nm and quantitative analysis on an agarose gel. For reliable
| + | |
| - | spectrophotometric DNA quantification, A260 readings should lie between 0.1 and 1.0.
| + | |
| - | Agarose gel analysis
| + | |
| - | We recommend removing and saving aliquots during the purification procedure
| + | |
| - | (samples 1–4). If the plasmid DNA is of low yield or quality, the samples can be
| + | |
| - | analyzed by agarose gel electrophoresis to determine at what stage of the purification
| + | |
| - | procedure the problem occurred
| + | |
When working with chemicals, always wear a suitable lab coat, disposable gloves, and
protective goggles. For more information, consult the appropriate material safety data
sheets (MSDSs), available from the product supplier.
■ Standard microbiological equipment for growing and harvesting bacteria (e.g.,
inoculating loop, culture tubes and flasks, 37°C shaking incubator, and centrifuge
with rotor and tubes or bottles for harvesting cells)
■ Centrifugation tubes or vessels with suitable capacity for the volumes specified in the
appropriate protocol.
■ Refrigerated centrifuge capable of ≥20,000 x g with rotor for the appropriate
centrifuge tubes or bottles
