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RNA Editing

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Title: RNA Editing


1
RNA Editing
  • Definition any process, other than splicing,
    that results in a change in the sequence of a RNA
    transcript such that it differs from the sequence
    of the DNA template
  • Discovered in trypanosome mitochondria
  • Also common in plant mitochondria
  • Also occurs in a few chloroplast genes of higher
    plants, and at least a few nuclear genes in
    mammals

2
Discovery of RNA Editing in Trypanosome
Mitochondria
  • Unusual Mitos. called Kinetoplasts
  • DNA
  • Maxicircles (22 kb in T. brucei), contains most
    of the genes
  • Minicircles (1-3 kb), heterogenous
  • Sequencing of genomic Mt DNA (Maxicircles)
    revealed apparent pseudogenes
  • Full of Stop codons
  • Deletions of important amino acids

3
Kinetoplast DNA from a trypanosome visualized by
EM
4
  • Where were the real functional genes?
  • Investigators generated cDNA clones to some of
    the kinetoplast mRNAs and sequenced them
  • Sequences were partially complementary to
    pseudogenes on maxicircle DNA
  • cytochrome oxidase
  • subunit II
  • the COXII DNA sequence above is missing 4 Us
    found in the mRNA
  • Called this Editing because it produced
    functional mRNAs and proteins from pseudogenes

5
Some genes are very heavily edited!
COXIII Cytochrome oxidase III From Trypanosoma
brucei
Lower case Us were inserted by editing. The
deleted Ts (found in the DNA) are indicated in
upper case.
Fig. 16.20
6
Editing Mechanism
  • Post-transcriptional
  • Guide RNAs (gRNAs) direct editing
  • gRNAs are small and complementary to portions of
    the edited mRNA
  • Base-pairing of gRNA with unedited RNA gives
    mismatched regions, which are recognized by the
    editing machinery
  • Machinery includes an Endonuclease, a Terminal
    UridylylTransferase (TUTase), and a RNA ligase
  • Editing is directional, from 3 to 5

7
Guide RNAs Direct Editing in Trypanosomes.
Editing is from 3 to 5 along an unedited RNA.
16.22
8
Editing Mechanism with the enzymes.
TUTase Terminal Uridylyl Transferase
From Fig. 16.25
9
Other Systems with RNA Editing
  • Land plant (C ? U) and Physarum (slime mold)
    mitochondria (nt insertions)
  • Chloroplasts of angiosperms (C ? U)
  • A few nuclear genes in mammals
  • Apolipoprotein B (C ? U)
  • Glutamate receptor B (A ? I (inosine))
  • Hepatitus delta virus (A ? I)
  • Paramyxovirus (G insertions)

10
Editing of Angiosperm Mt RNAs
  • Most RNAs are edited
  • Most events are C ? U but also U ? C
  • Preferential editing of coding regions, but
    introns and untranslated regions are also edited
  • Editing produces translatable RNAs, and restores
    conserved amino acids (i.e, functional proteins)

11
Editing of Oenothera mitochondrial RNAs
Determined by comparing sequences of cDNA copies
of mt RNAs with the corresponding genomic gene.
12
Possible mechanism for plant Mt editing
Deamination of cytosine (to uracil) by a cytidine
deaminase
NH2
O
N
N
H20
O
O
N
N
Cytosine
Uracil
13
Plant mt RNA Editing Mechanism (cont.)
  • Cytidine deaminases are known, and in fact one
    is involved in ApoB editing in mammals.
  • How are editing sites recognized?
  • No guide RNAs have yet been found in angiosperm
    mitochondria

14
Editing of Apolipoprotein B in Mammals
  • Large nuclear gene
  • Editing is C6666 ? U6666 in exon 26 of the 14 Kb
    mRNA
  • This creates a Stop codon, producing a truncated
    form of the protein
  • - both forms circulate in blood but have
    different functions
  • - the long form is endocytosed via the LDL
    receptor the short form is not

15
Molecular Consequences of Editing ApoB pre-mRNA
Splicing precedes editing
Produced by Unedited mRNA
Produced by Edited mRNA
16
Editing of Apolipoprotein B The Editosome
  • A cytidine deaminase activity is involved
    apobec (apoB mRNA editing enzyme catalytic
    subunit)
  • Another protein, ACF (apobec complementation
    factor) is also required
  • Both recognize sequences flanking the C to be
    edited

17
Mechanism of A to I Editing
  • dsRNA-dependent adenosine deaminase (ADAR)
  • converts A ? I in 2 Glut Receptor B exons
    (changes the amino acids, I read as guanosine
    during translation)
  • recognizes secondary structure around site to be
    edited
  • requires intron and exon sequences - acts on
    unspliced receptor pre-mRNA
  • has dsRNA binding domains as well as a catalytic
    center similar to the cytosine deaminase

18
  • 2 online references for more about nuclear RNA
    editing
  • Davidson, N. (2002) The Challenge of target-site
    specificity in C ? U editing. J. Clinical
    Investigation 109 291-294
  • Maas, S. and A. Rich (2000) Changing genetic
    information through RNA editing. Bioessays 22.9
    790-801
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