FYI: I m attached to research lab under the Cellular and Molecular Research division. My lab focuses on gene structure and expression.
I was assigned to do a project to prevent 2 proteins from interacting to prevent tumorigenesis.
Throughout my SIP, I did different things everyday unless I don’t get any expected results and need to redo. My work rotates around Mbio, CellBio, MCT and Biochemistry. I am going to focus on DNA preparation in my discussion here. I am supposed to isolate the DNA I clone from the host cells that I had transformed.
There are three types of DNA prep for plasmid isolation: maxi-, mini, midi-prep.
Below are differences between these 3 prep works:
As I only did the maxi- and miniprep, I cannot comment more on midiprep.
Maxiprep:
-large scale DNA preparation
-Quantity of DNA eluted: 500ug/ml- 850ug/ml
Steps and reagents involved:
-Uses cultured cell clones in 250ml of LB media
- Requires centrifugation at 4۫C
- Requires a big Maxi- column to bind DNA, a dish to collect flow through that pass the column for disposal and a Du-pont tube for DNA elution
- Steps are lengthy and more buffers are involved like W8 (wash buffer), E4 (elution buffer), 70% ethanol for precipitation, TE buffer for resuspension and Equilibration Buffer (EQ1) to wet the column before draining any solution
- Drain through column by gravity flow
- Principle is lysis, bind and wash DNA, precipitation and elution.Details of the protocol can be found in www.invitrogen.com under PureLink™ HiPure Plasmid Filter Purification
Miniprep
-Small scale DNA preparation
-Quantity of DNA: up to 40ug/ml
-Steps and reagent involved:
-Uses cultured cells in 4ml of LB media
-Only requires a normal centrifuge
- Only requires a normal spin column to bind DNA and 2ml Wash tube to elute the DNA and for flow through collection
-Involves lesser steps and buffer and column work by centrifugation to bring the solution down.
- Principle works by alkaline lysis of the host cells, bind, wash and elution purified DNA.
- Details of the protocol can be found in www.invitrogen.com under PureLink™ Quick Plasmid Miniprep Kit
Midiprep
-Middle scale DNA preparation
-Quantity of DNA: 100-350ug/ml
After the prep for our DNA purification, I need to do a quantitation of DNA content using a spectrophotometer to check is there sufficient DNA for the following steps of the project. Quality of DNA is also monitored. DNA with ratio measured at 1.6-2.0 are considered pure and good quality. Sometimes, ratio may not be quantitated by the spectrophotometer if the concentration is too low. The Miniprep is done before maxi prep so that we can prepare our large amount of DNA with the correct sequence based on the sequence results of the clone from miniprep. We quantitate the DNA in miniprep for sequencing reaction to monitor if the DNA cloned has the right sequence so that we can proceed on our project. 1 ug/ml is sufficient.
For maxiprep, we check the concentration of DNA to see if there are enough for in vitro translation for translating DNA to proteins in the next part of project .
Running a gel with the same aliquot of DNA can confirm the quality of DNA based on comparison of the intensity of the bands to make sure the measurement from the spectrophotometer is accurate. DNA might be contaminated with RNA, proteins and carbohydrates which can be determined by the quality ratio of the DNA and confirmed again using the gel.
I hope u all understand what I said and dont hesitate to ask. Thanks.
Ai Tee
0503160D
TG01
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15 comments:
Hello Ai Tee
For the 3 types of DNA pre for plasmid isolation, what are some of the factors that may affect each of them? Thanks
Ci Liang
TG01
hey gail~
Is the miniprep done to just assess whether the DNA sequence is correct before performing the Maxiprep?
Thanks! =D
Charmaine Tan
TG01~
Hey there! Glad to see something on genetics - feel so lost when i see haem everywhere!
Anyways, how do you prevent 2 proteins from interacting with each other once you've translated them?
Also, prior to this you mentioned DNA cloning. if so, was the insert(s) provided or need to amplify by PCR or cut from another vector? (if they have stock).
Lastly, how many clones do you normally screen and do you use restriction digestion to do so or just colony PCR? In my lab, typically screen about 20 clones per plate.
P.S Ligation you use 16 degrees overnight or the rapid type?
Sorry for the mulititude of questions!
- Debra, TG02
- Debra
Hey-lo
Im just going to ask you a simple question in comparison with what I am doing for my MP.
We run gels to confirm positive products of our PCR reactions based on comparison of the intensity of the bands to DNA ladders.
Can you tell me what type of loading dye you use, whether you use a 100bp ladder or 1000bp ladder and if possible why do you use them. Are they better in any way?
Thanks,
Azhar TG01
Hi Galye
Can I ask you, if the DNA concentration is too low to be quantitated by spectrophotometer, what do you do?
Eugene Wong
TG02
hi Gail...
I just wanna you, issit important to do miniprep before maxiprep??
Or it can be done individually??
and basically the difference btw these two methods is the duration to complete the followong tesT??
Vinodhini
TGO1
hi ci liang,
sorry for taking to reply so long.. i don understand what u mean by factors affecting them? u mean affecting the choice of selecting which prep to be done?
hi char,
no.. as long as you quantitate them and its enough for use, u can use the pure DNA directly in other downstream applications such
as sequencing, PCR, cloning and
transformation. as for me, i do the sequencing reaction to check my DNA b4 my maxiprep.
hi debra,
e.g: A is the one that will activate B to cause tumor
so we prevent the 2 proteins by introducing smth with similar structure as B to bind to A so that we block A from activating B.
the insert was provided but i cut them with restriction enzyme to linearised the plasmid and then amplify by PCR becuase efficency for circular DNA is low.
for the cloning part, the number of clones to select depends on the digest u do. if single digest, we need more clones as the insert may be orientated in the wrong direction inside the vector or in the direction we want. therefore, we have 50% chance of getting the correct clones. i seen the ppl there doing 8 clones for single digest. for my double digest, because the insert can only be orientated in one direction we will have 100% chances of getting the right clone. we inoculate 4 clones as 1 or 2 clones may differ due to cloning artifacts. the max to inoculate your clones is 20.
i did my ligation the rapid type i tink.. coz i incubate them for 1hr at room temp.
hello azhar
i use a 1kb DNA ladder. i use a 10x loading dye. the DNA ladder is chosen as my DNA is only 600bp in size. the DNA ladder is chosen depending on the DNA u run.
hi eugene,
if DNA concentration is low, it means that we lose alot of our DNA during our plasmid purification. if so, we troubleshoot and see what is the problem and repeat the experiment once again as long as we got enough DNA. for e.g: i did a mistake by using 1.5ml tube instead of 2ml recommended in the protocol. therefore, the DNA is not eluted well as the solution when passed into the spin column did not flow well through the column after spinning and DNA might not bind to the column and get discarded with the flow through.
hi vino,
ya.. its impt to do the miniprep to check the sequence of DNA. if u want to do maxiprep and check the sequence and u find that the sequence is wrong, it will wasting resources and time. miniprep can be done within 2 hrs, if fast enough as the protocol estimate is 45mins. maxiprep needs around half a day and everything is in large scale and require large centrifuge and i need to walk to other labs to use it. u need large bottles, columns and filters which is more tedious and time consuming than miniprep. more buffers are also involved and steps are lengthy. basically, the two prep differ in the quantity of DNA eluted, the buffers and column used and of course the duration . in miniprep, we use a small column which we use to use in MBIO and the solution flow when we spin them but in maxiprep, we use large column and they need to flow by gravity which is slow.
hello
sorry if i did not phrase my qn properly. Actually i m trying to ask while doing the DNA pre, is there any factors that can affect it? Thanks again
Ci Liang
TG01
Your blog keeps getting better and better! Your older articles are not as good as newer ones you have a lot more creativity and originality now keep it up!
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