20th Feb - Splicing, In Vitro and the chemical reactions Flashcards
What are the two major problems for establishing splicing reactions in vitro?
Getting a defined piece of RNA
Adding the RNA splicing system
What was the solution to producing a defined piece of RNA?
Using T7 RNAP
What was the solution to getting the RNA splicing system in vitro?
Injecting Xenopus oocyte nuclei however this was of limited use biochemically
Now use cell extracts commonly from HeLa cells then put them into a lower ionic strength buffer
How is a nuclear extract made?
By putting nuclei in hyperosmotic medium, causing competition between the proteins in the nucleus, causing all nuclear proteins to leave the nucleus except histones
Outline Krainer’s experiment which showed that mRNA is made as part of a 2-step reaction
Took out samples at varying times and analysed the products on a gel
Found that the pre-mRNA yield declines with time
Found that the mRNA yield increases with time but at a different rate
What led to the hypothesis that the intermediates of splicing were branched or circular?
They ran differently on different strength gels, they appeared to gain Mw
How was it identified that splicing intermediates were lariats?
RT PCR with 2 primers
- Circular would lead to one band on the gel
- linear would lead to two different weight bands
- -> Primer 1 strand was very short
Thus could it be branched? Lariat or Y-shaped?
- -Cut with RNase H, which cuts where an oligo is branched
- Y shaped would create 2 molecules
- Lariat would create 1 molecule
- -> 1 molecule therefore the intermediate was a lariat
How did was the branch site mapped to within a few NTs?
- Used RNase H
- Added NT’s at various points along the intron and mapped the linear piece
- Cleavage within the loop would produce an aberrantly moving Y shaped molecule –> huge shift in mobility. When cleave at the branch point –> a straight full intron
- From this they used the specificity of ribonucealses to show the branch point, using labelled GTP
–> Cut with T1 and T2 gave two radioactive G and 1 radioactive A
How was the branch site identified to 1 NT?
RNase T2 digests all RNA to Np except branchpoints which end up as X (pYp)(pZp) (where X is the branchpoint and Y is the linked base and Z is the base after)
A phosphatase can then be applied to remove the end phosphate
- RNA was labelled with individually radio-tagged NTPs
- -[alpha32P] ATP –> no labelling
- -[alpha32P] CTP –> labelling
- -[alpha32P] GTP –> labelling
- -[alpha32P] UTP –> no labelling - Y and Z = G and C
- Thus the branch is A
How was it identified that step 1 of splicing was a transesterification?
Replaced 1 oxygen with sulphur making the phosphate group chiral.
A transesterification would cause an umbrella conversion
