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PCR product appear two close band in my gel - (May/22/2010 )

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The exact band size of my PCR that i want is around 305bp...but i am getting another band which is 20-30bp less than the band size that i should get. I have 2 band in my PCR product!!!I don't know what reason that cause this and anyone here can explain to me? Please!

-Fhannan-

Fhannan on May 22 2010, 08:05 AM said:

The exact band size of my PCR that i want is around 305bp...but i am getting another band which is 20-30bp less than the band size that i should get. I have 2 band in my PCR product!!!I don't know what reason that cause this and anyone here can explain to me? Please!

It means, that u have one specific and one nonspecific band in ur PCR? Did u try to optimize it? To increase annealing temperature, or decrease primer concentration, or to use some additives? If so, isnt it some contamination there (DNA from other species for example)?

-galileo-

Thanks for the answer,
I am doing two reaction for 2 fragments, the PCR product for one fragment is showing two bands, while the other shows one specific band only, so i guses it is not contamination problem that we are talking about here, regarding the annealing temp i am using two primers one with 59.4 C, the other is 55.3 i am running my reaction with 52C annealing temp with 0.2uM final primer conc. do these conditions seem fine?

-Fhannan-

Fhannan on May 22 2010, 09:40 AM said:

Thanks for the answer,
I am doing two reaction for 2 fragments, the PCR product for one fragment is showing two bands, while the other shows one specific band only, so i guses it is not contamination problem that we are talking about here, regarding the annealing temp i am using two primers one with 59.4 C, the other is 55.3 i am running my reaction with 52C annealing temp with 0.2uM final primer conc. do these conditions seem fine?

Did u try temperature gradient? U can try also BLAST, to verify your primers. Do u have some PCR troubleshooting? It can helps u, if u dont know what to do (for example this one: http://www.abgene.com/downloads/PCR_Troubl...ting_Guide.pdf).

-galileo-

Perhaps DNA from a heterozygous organism?

-hobglobin-

Its Human DNA samples...

-Fhannan-

Have you done a check for potential secondary binding sites? Is it possible to raise the tm of the 55 degree primer? Even adding 1 base to bring the Tms closer will mean you can run with a higher annealing temp, and reduce the risk of mispriming. Also, what are you using?

-swanny-

Hello,
i am using 1.5mM Mg+2 conc. i have been trying to optimize the reaction by increasing annealing temp to 55 and 58 and decreasing primer and DNA template with no luck!

-Fhannan-

Did you still get the two bands at Ta=58ºC?

Try increasing the Ta even further. If you continue to see the two bands, at the same brightness, then it might be due to a specific, second target region in the genome (check this by BLAST or in-silico PCR). Alternatively there might be a heterozygous deletion in your DNA sample.

You could re-design your primers and/or cut out, gel-purify and sequence your bands. At least you'll then know for sure where this second product is coming from.

-jamessmith01-

I checked by blast that only one fragmet should be amplified..
I have tried to optimize the protocol, in all cases I got either no amplification or unspecific amplification in 2-3 banding pattern. I tried to use the following ranges of :
- 0.5, 1, 1.5, 2, 3ul of primers
- 50ng (0.2ul), 100ng (0.5ul), 300ng (1.5ul) of DNA
- 5ul, 6ul 6.7ul of 10xbuffer with mgcl2 which gives the following final Mg+2 conc. respectively 1.5mM, 1.8mM, 2.1mM
I carried out the reaction under 55C which I saw the it gives better bands comparing with 52C, 58C, 62C
Are there any suggestion that could improve the results, I attach a gel photo that shows the unexpected bands

The Std protocol is as follow
dNTPs 1ul (200uM)
Primers 2ul (02uM)
10x buffer 5ul
DNA 1ul (5-100ng)
Enzyme 0.5ul
dH2O 40.5ul
Total 50ul



Primers annealing temp is
45F 59.4 C
45R 55.3 C

-Fhannan-
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