丁香实验_LOGO
登录
提问
我要登录
|免费注册
点赞
收藏
wx-share
分享

Screening of cDNA and genomic libraries

互联网

668

 

 
<center>  </center> Choice of bacterial strain:

The bacterial E. coli strains we use when plating out cDNA and genomic libraries are normally LE392 and NM538, but some times we also use XL1-blue cells.
 
 

  • Streak out bacteria on a LB plate. Pick a single colony and transfer to a flask with 50 ml LB. NB! remember to add maltose to the LB, 0.2% final concentration. Grow over night.
  • Spin down cells in a 50 ml Falcon tube and resuspend in 20-25 ml 10mM MgSO4 . The bacteria can be stored at 4 C for up to one month, but if you are using the bacteria to check the titer of the library or to plate out the lambda library (primary plates), ALWAYS use fresh bacteria.
Checking the titer of the library:
 
  • Make a dilution series of the library. Depending on the titer of your library, normally around 108 - 109 pfu/ml, take out 10 ul of the library stock solution ul and transfer to 990 ul SM solution, this will be the "107 " stock solution which you normally plate the library from. Make a 1/100 dilution of the 107 stock, (105 mix), a 1/100 dilution of the 105 mix (103 mix), and a 1/100 dilution of the 103 mix (101 mix).
  • Transfer bacterial cells (ex. LE392), to 3 eppendorf tubes, 100 ul in each. Add 2 ul of the 105 mix, 2 ul of the 103 mix, and 2 ul of the 101 mix. Incubate for 15 min. at 37 C to let the phage particles adhere to the E. coli cells.
  • Melt the top agarose in microwave oven, transfer 3 ml to 15 ml tubes.
  • Transfer the phages and cells to the top agarose, 3 ml in a 15 ml. tube. (The tube with topagarose is kept in a water bath at 50 C). Invert the tube a couple of times and pour the top agar on a lambda plate. Wait until the top agarose has solidified and incubate the plates at 37 C until you see the plaques.
  • Count the plaques and calculate the titer of the library.
    • Top agarose, 500 ml:
       
      • 5 g. bactotryptone
        2.5 g NaCl
        3.5 g agarose
        add MgSO4 to a final cons. of 10 mM
    • Lambda plates, 1 liter.
       
      • 10 g. bactotryptone
        5 g. NaCl
        14 g. agar.

 

Plating out the library:
 
 

Example for plating out 12 plates, 300.000 pfu.
 

    It is important to use fresh bacterial cells. We normally plate out from 10-15 plates (140 mm) depending on the library. That is from 300,000 to 500,000 pfu.
  • Take out 3.6 ml of E. coli cells (grown with 0.2 % maltose), and transfer to 15 ml tube.
  • Add 300,000 pfu from the library, x ul.
  • Incubate 30 min. at 37 C.
  • Transfer 300 ul of phages / cells to 7 ml topagarose (tubes with topagarose is kept at 50 C). Invert the tube a couple of times and pour the topagarose over the lambda plate, 140 mm.
     
    • It is important that the lambda plate is "dried out" a bit before you use them. Pouring the topagarose onto a "wet" newly made plate can give problems when you take filter lifts later.
       
  • Plate out all the phage, (the 11 remaining plates). Let the top agarose solidify and incubate the plates at 37 C.
  • Watch the plates carefully when the bacteria grow. cDNA libraries are normally much "faster" to produce plaques, and you can normally see them after 4 hours. Wait until the plates are almost confluent. That takes 5-7 hours with cDNA libraries and 6-10 hours with genomic libraries.
  • When the plates are ready you can store them at 4 C over night. If the plates are almost confluent you might expect some diffusion of phages but that is normally not any problems.
     
Taking lifts of the plates, (transferring the lambda phage to nylon membranes).
 
 
    We normally use Amersham Hybond N filters / membranes. They are robust and can be re-screened many times. When you take lifts of the primary plates, the complete library, we recommend that you take duplicate lifts. For high stringency screening, (hybridization and washing at 65 C), this may not be necessary but for low stringency screening it is a must.
     
  • Label the filters thoroughly. Place the filter on top of the top agarose for about 1-2 min. Then using a needle mark the filter with needle holes. (These holes are necessary when you later align the filters and exposed films). We also mark the needle holes at the back side of the lambda plate with a marker. This makes it easier to align the exposed films against the plates.
  • The duplicate filter is placed on the top agarose for 2-5 min., and marked similarly as the first filter.
  • Let the filter dry. The lambda phage is now transferred to the filter.


    Denaturation solution:   1.5 M NaCl, 0.5 M NaOH

    Neutralization solution: 1.5 M NaCl, 0.5 M Tris-Cl pH 8.0
     

  • Soak the filter in denaturation solution for 2-5 min. Transfer the filer to 3M paper where it partially dries up.
  • Soak the filter in neutralization solution for 5 min. Transfer the filer to 3M paper where it partially dries up.
  • Wash the filter two times in 2 X SSC.
  • Let the filters dry.
  • UV fixate for 1-2 min. (the time depends on the strength of your UV transilluminator).
  • The filters are ready for use. Before use they should be stored in a dry place at room temp.
    Keep the library plates good wrapped in a plastic bag at 4 C to avoid that they dry out. The library can be kept at 4 C for months, but the titer will gradually decrease.


 

Probe labeling:
 
 

    It is normally enough to label 20-50 ng probe, and use approx. 50 uCi 32 P alpha dCTP. Any kind of random labeling kit will work; just follow the manufacturer recommendations. After the hybridization we normally clean up the probe on a nick column, (Sephadex G-50 size exclusion column from Pharmacia). This normally gives a clean probe eluted in a 500 ul TE. Before you use the probe remember to boil it!! (You need a single stranded probe in the hybridization). Boil the probe for a couple of minutes and place it on ice until you add it to the hybridization solution.
Filter Hybridization:
 
 
  • Pre-hybridization:


    We always do a 1-2 hour pre hybridization before we start the real hybridization with the probe. Our pre hybridization buffer is more or less the same to the one you find in Maniatis.
     

    • 6 X SSC, 5 X Denhards, 0.5 % SDS, 10 ug/ml salmon sperm DNA.
       
  • Pre-hybridization is normally done at 60 - 65 C, in a water bath with shaker.
     
  • Hybridization:


    We normally do the hybridizations in a glass dish / glass beaker, using a water bath to control the temperature. The hybridization volume can be from 20-100 ml. The larger the volume the longer you need to run the hybridization. One to two days is normal if the volume is above 50 ml. Over night hybridization is enough if the volume is less than 50 ml.
    Hybridization solution:
     

    • 6 X SSC, 0.5 % SDS, plus the 32 P labeled probe.
       
  • Boil the probe before you add it to the pre-warmed hybridization solution, (approx. 60 C).
  • Pour off the pre-hybridization solution and add the probe/hybridization solution.
  • Seal the hybridization "container", (a sealed plastic bag, or hybridization beaker or a Hybaid glass, or whatever you might find to do the hybridization in).
  • Hybridization temperature depends on your probe and what you are screening after.
     
    • High stringency screening: 65 C.
    • Medium stringency: 55-62 C.
    • Low stringency: 50-55 C.
    After the hybridization pour the probe into a 50 ml tube and put it in a -20 C freezer. Shield the probe. The probe can be reused a couple of times.
     

 

Washing of the filters:
 
 

    We normally wash the filters in SSC / SDS solutions after the hybridization is done. The washing solution and temperature depends on your probe and stringency conditions.
     
    • High stringency wash: 0.1 X SSC, 0.1 % SDS, at 65 C.
    • Medium stringency wash: 0.5 - 1.0 X SSC, 0.1 % SDS, at 55-62 C.
    • Low stringency wash: 2 X SSC, 0.1 % SDS, at 50-55 C.
       
  • Normally you wash the filters 2 - 3 times in a volume of 200-300 ml. Check the activity of the filters with a Geiger counter. Too high activity normally means that the background signals are high. The activity shall normally be "low", that's unless you have 10-100 of positive clones pr. filter.

After you have developed the film you normally see a faint contour of the membranes together with the dark spots of the positive clones. If you do not see the contour of the membranes you will have to make some radioactive ink, (S35 or P33 ) or use "a Stratagene marker" and label the Saran wrap you have wrapped around the membranes. If you can see the contours of the membranes, put the developed film on top of the membranes and align the film so they match. (This is best done on a light table, the needle holes in the membranes is also easier to spot that way). Mark all the needle holes onto the film with a marker. Find the lambda plate which corresponds with this membrane and align these marks with the marks on the plate. If you have done a good job they should overlap 100%. You are now ready to pick a positive clone...and probably 10-100 other neighbor clones. To be sure you do not miss the clone use the back of a pasteur pipette to pick the clone. If it i difficult to get the plug with the positive lambda loose try to suck it loose. (Try not to act like a vacuum cleaner you might end up swallowing it, no joking..). Place the plug in 1 ml of SM solution. Let the plug soake overnight. If it is a fresh library you have to make a dilution, 1/100 is normally OK. If it is a old library (more than one year), the titer has normally fallen so low that you can plate out the phage without diluting it. (cDNA libraries often have higher titers than genomic libraries).

Transfer 100 ul of LE392 (or the cells you used when you plated the library) and add 2 ul of the lambda phage. Incubate for at least 15 min at 37 C, add the mixture to a 12 ml tube with 3 ml top agarose, invert the tube a couple of times and plate it out on a 82 mm. lambda plate. Incubate the plates at 37 C until you have a good plaque size. The secondary plates are now ready for lifts.

These next steps (taking lifts of the secondary plates, hybridization and all that) are similar to the ones described above.

If you are able to pick clean plaque pure phage from secondary plates you are lucky. If not start over again, pick the positive clones but this time make sure you plate out less phage on the plate. You should try to plate out less than 100 pfu on the tertiary plates.

When you have picked a plaque pure clone from a lambda ZAP library you are ready to roll, (just use the manufacturer descriptions how to do the excision of the bluescript plasmid). If you are screening a genomic library however (a lambda FIX vector or similar) you should be 100 % sure you have a plaque pure clone. If you start up running lambda preps with a clone which is not 100% clean you may end up with some nasty surprises. To be sure that does not happen you should do a last check, a "plaque pure screen", where you plate out the clone you think is plaque pure and re-screen it. From the plate where all the clones are positive you pick your master clone! Make a plate lysate from this clone. That is: plate out a confluent plate from this clone. Add two ml of SM to the confluent plate and place the plate on a rotary shaker for a couple of hours. Transfer the phage solution to a eppendorf tube. Add a couple of drops of chloroform to the tube and store it at 4 C.

    Wrap the filters in Saran wrap, and put them in a film cassette. You get the best results if you have screens in the cassette. Leave the cassette in a -20 C freezer for 1-2 days. Develop the film, and if you have done everything right and you library is good, you should have some positive clones to play with.

 

提问
扫一扫
丁香实验小程序二维码
实验小助手
丁香实验公众号二维码
扫码领资料
反馈
TOP
打开小程序