Multimerization Troubleshooting: No Luck in 2-3 Weeks

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The discussion centers on challenges faced in creating multimers from oligonucleotides. The user has attempted the process for 2-3 weeks, following steps that include annealing oligos, phosphorylating the 5' ends, and ligating overnight, but only achieved dimer formation when analyzed on agarose gel. Key issues identified include the possibility of inefficient ligation reactions or the formation of circular DNA molecules instead of linear multimers. It is suggested that increasing the DNA concentration in the ligation reaction could enhance the likelihood of successful ligation with new DNA molecules. Additionally, the size of the oligos used is noted as a potential factor; smaller oligos may lead to more circular products. The user seeks established protocols to address these issues effectively.
karthik3k
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Multimers :((

I have been trying this thing for past 2-3 weeks with no luck :((

:cry:

I am trying to make a multimer from an oligo.
This is how i did:
- Annealed the oligos
- Phosphorylated the sample (5' ends)
- ligated o/n

when i ran it on agarose it shows only a dimer. what can be the reason ?
any ideas ?

Should i use some different protocol ??
 
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When I did ligations, I could see a ladder. My fragment was in a vector, which I excised with restriction enzymes. The result is sticky ends which ligate much better than blunt ends.

So either your ligation reaction is not efficient, or you are making circular DNA molecules. The get more linear product, you should ensure that the concentration of DNA in your ligation reaction is quite high. That way the DNA is more likely to come across a new DNA molecule to ligate to, than it is to its own free end. Another problem I see is that you use very small oligos. Mine were 100 bp, so the ends are further apart, thus less circular products.
 
k.

do u have any established protocol for this kinda problem ? :confused:
 

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