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RNA Isolation (objectives)

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The lysate is diluted with ethanol and applied to a glass or like RNA binding matrix. proteins and other contaminants are removed by subsequent washes The total RNA ... – PowerPoint PPT presentation

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Title: RNA Isolation (objectives)


1
RNA Isolation (objectives)
  • Understand why we isolate RNA
  • Know ways of inactivating RNases
  • Understand the basic principals in isolating
    total RNA and mRNA

2
Why isolate RNA?
  • Northern Blots for looking at gene expression
  • As a source for cDNA libraries
  • RT-PCR
  • Nuclease protection assays

3
Extraction of RNA (important factors)
  • All solutions need to be treated to remove RNases
  • diethyl pyrocarbonate treatment for non amine
    solutions
  • protein inhibitors of RNases (RNasin)
  • controlling RNase activity
  • all glassware, plasticware, etc needs to be
    treated by backing at 180C for 8hrs (glassware)
    or washed in chloroform (plasticware)
  • An alternative treatment is washing in DEPC
    followed by autoclaving
  • disposable gloves
  • be paranoid
  • RNase Zap

4
Extraction of RNA (important factors)
  • Tissue source of RNA
  • Preservation of RNA integrity
  • liquid nitrogen
  • RNA later RNA stable in tissue stored for up to
    1 day at 37C, 1mth at 4C and indefinitely at
    -20C.

5
RNA Later
6
Extraction of RNA (manual)
  • Suspension of cells in RNA homogenisation buffer
  • NaCl, MgCl2, Tris, Nonidet P-40, DTT, RNase
    Inhibitor
  • Add RNA extraction buffer
  • Tris pH 8, EDTA, NaCl, SDS, Proteinase K
  • 37C/30min
  • Phenol/chloroform extraction
  • Precipitate RNA
  • Resuspend and add RNase free DNase I, RNase
    Inhibitor, MgCl2 and DTT (37C/60min)
  • Extract in Phenol/chloroform

7
Extraction of RNA (manual)
  • Precipitate RNA
  • resuspend in TE
  • There are other methods which use a guanidine
    thiocyanate which effectively lyses cells and
    inactivated ribonucleases
  • Trizol is another type of isolation reagent

8
Extraction of RNA (Column)
  • Qiagen and Ambion make column based kits for
    isolation of total RNA
  • The cells are disrupted in guanidine thiocyanate.
  • The lysate is diluted with ethanol and applied to
    a glass or like RNA binding matrix.
  • proteins and other contaminants are removed by
    subsequent washes
  • The total RNA is eluted

9
mRNA isolation
  • Only about 3 of total RNA is specific message
    (mRNA). Most is 28S and 18S
  • eg in 5mg of tissue about 10ug of RNA is present
    of which 0.3 ug is mRNA, a rare message accounts
    for 10fg-10pg in total, and a moderately abundant
    message 300pg
  • How can we isolate such small amounts of message?

10
mRNA isolation
  • We utilise the feature of mRNA, ie the poly A
    tail
  • Using a column containing a synthetic
    oligonucleotide oligo(dT) attached
  • hybridise the mRNA to the oligo(dT) and wash away
    the remainder
  • Elute the mRNA by hot buffer
  • Usually we do two rounds of purification
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