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pcr cloning

boa

By boa
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boa

boa

Posted
Posted (edited)

I have no clue where to start but I think it is safe to say that my forward primer could be TAC and my reverse primer TTA (complementary sequences of the start and stop codon) but I dont know what to do after...the problem seems very overwhelming to me! I would like someone to provide me some hints to tackle this!

Thanks everyone!Thank you for your help!

 

Question :

Write the sequence of two oligonucleotides that will allow you to clone the coding region of gene x

in the vector pQE60 using PCR . The coding sequence must be in frame with the ATG of the vector. The histidine tag must be present

at the C-terminus of your recombinant protein. The oligos must be as short as possible but must

hybridize with 20 nucleotides of the template sTrand. The start and stop codons of gene X are

underlined.

 

Coding sequence of gene X

GTCGATCAAT ATGGAACATG TTTACTCCAA ACCACCGCAC ACCAATTATG

GAAACCAAGC CGGAAAAGAA TTCCGGTGGA GAGCGAAAAA AAAGGATTCC

GAATCGTGAA CTGCCAAAAA CATTTTGAAG CCAACGATTC CGACGTCATC

CTCGCCACCC TAGCTAAATC AGGCACCACT TGGTTAAAAG CTCTTCTCTT

TGCTCTCATT CACCGACACA AGTTCCCAGT TTCTGGCAAG CATCCTCTTC

TGAAACAGCA GTAGCAGCGT TTAAAGGGAA GTTTATT

 

Oligo #1 5' ________________________________________…

Oligo #2 5' ________________________________________…

 

Nco1 = CCATGG BamH1 = GGATCC BglII = AGATCT HindIII = AAGCTT

 

pQE60 (RBS)CCATGGGAGGATCCAGATCT(blackbox) TAAGCTTCCGCATAATTAGCTGAG

Additional Details

The start and stop codons of gene X are the first ATG and the last TAA

 

underlined in vector pqe60: the first ATG

 

 

----

 

I have no clue where to start but I think it is safe to say that my forward primer could be TAC and my reverse primer TTA (complementary sequences of the start and stop codon) but I dont know what to do after...the problem seems very overwhelming to me! I would like someone to provide me some hints to tackle this!

Thanks everyone!

Edited by boa
CharonY

CharonY

Posted
Posted

Check out the requirements of your primer. First, it has to hybridize with 20 bp. So the minimal length is 20. You do need to add a His-Tag on the C-terminus (which primer would that be?). So far you offered 3 bp for each primer only.

In addition you may want to think about compatibility with the vector (though you can always blund-end ligate).

boa

boa

Posted
  • Author
Posted

Check out the requirements of your primer. First, it has to hybridize with 20 bp. So the minimal length is 20. You do need to add a His-Tag on the C-terminus (which primer would that be?). So far you offered 3 bp for each primer only.

In addition you may want to think about compatibility with the vector (though you can always blund-end ligate).

 

Ok, so I tried to make primers according to gene X...

so for the forward primer(oligo 1) I have : 5-ATGGAACATGTTTACTCCA-3

and for the reverse primer (oligo 2) : 5-TTAAACGCTGCTACTGCTGT-3

 

Am i doing this right? Also, how do I include the his tag? I dont understand what the c terminus thing is about...

Thanks!

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