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TRANSCRIPTION
DR. Vishnu Kumar
PROFESSOR AND HEAD,
DEPT.OF BIOCHEMISTRY
MPTMC, SIDDHARTH NAGAR
COMPETENCY NUMBER BI 7.2
LEARNING OBJECTIVES
After completion of this lecture learner should
be able to define/ Describe:
 Synthesis of RNA from DNA template
 The primary transcript
 DNA dependent RNA polymerase
 Steps of RNA synthesis
 RNA Classes
 Post Translational Modification
Transcription
Synthesis of RNA from DNA template.
The sequence of ribonucleotides in RNA molecule is
complementary to the DNTPs in one strand of DNA
called the template strand or sense strand.
The other strand is called the coding strand or anti
sense strand because it is identical to the RNA except
U for T.
Direction & enzyme involved
 The information in the template
strand is read in 3’ 5’ direction &
the RNA is synthesized in 5’  3’
direction.
 Enzyme involved  DNA dependent
RNA polymerase. The enzyme
attaches itself at a specific on the
DNA, the promoter site on the
template strand. This is followed by
initiation of RNA synthesis.
The primary transcript
 hnRNA generated by RNAP is
promptly capped by 7-methyl
guanosine tri phosphate, which will
eventually appear in the mRNA.
hnRNA contains both introns and
exons.
 The cap is necessary for protection of
mRNA from the action of 5’
exonuclease, also for recognition of
mRNA by the ribosome
DNA dependent RNA
polymerase
 in E coli it exists as a core molecule
having 5 subunits. 2 α, ββ‘ w. The
core RNAP utilizes a protein factor
called sigma factor.
 Core enzyme + sigma factor = Holo
enzyme.
Steps o RNA synthesis
 Initiation binding of holoenzyme to
the template at the promoter site to
form the initiation complex. This is
the closed complex. By sigma factor
there is unwinding of 2 DNA
strands. open complex.
 Binding is followed by a
conformational change of the RNAP.
Initiation Steps continued
 First nucleotide usually a purine
associates with the β subunit of the
enzyme. This becomes the 5’ of the
mRNA.
 In the presence of four RNTPs the
RNAP moves to the 2nd base in the
template.
 Sigma factor is released.
Initiation
 The enzyme polymerizes the
ribonucleotides in a specific sequence
that is dictated by template strand
and interpreted by Watson and
Crick’s base pairing rules. PPi is
releases at every step.
 A purine ribonucleotides is usually
first polymerized into the RNA
molecule.
Elongation
 Unlike DNAP, RNAP does not require a
primer and does not have proof
reading activity.
 RNAP has unwindase activity which
causes local unwinding of the DNA
double helix.
 As the RNAP pushes its way between
the strands it creates a +ve super
coiling ahead and - ve super coiling
behind it. Which are released by DNA
gyrases and topoisomerases
Termination
 Two types ‘ rho’ dependent and ‘
rho’ independent.
 ‘rho’ dependent here termination is
signaled by a sequence in the
template strand of the DNA molecule
(CA rich region) called ‘rut’ (rho
utilization) a signal that is recognized
by rho factor.
 Rho protein has an ATP dependent
helicase activity.
Rho independent
termination
 The RNA transcript must be able to
form a stable hairpin turn that slows
down the progress of RNAP. The
hairpin turn is complementary to a
palindrome sequence
 Following the hairpin turn the RNA
transcript must have a string of ‘U’ s.
the A=U bonding is weak which
facilitates its separation from the DNA
strand.
Termination
 After termination the core enzyme
separates from the DNA template.
 With the assistance of another sigma
factor the core enzyme recognizes
another promoter at which the
synthesis of a new RNA molecule
commences.
Transcription of eukaryotic
gene
 Far more complicated process than
that in prokaryotic gene.
 In addition to RNAP recognizing the
promoter region and initiating RNA
synthesis , a number of transcription
factors bind to distinct sites of DNA.
 There are 3 classes of RNAP in the
nucleus.
RNAP – classes
 RNAP1 synthesizes the 45S
precursor of r RNA (5.8s, 18s, 28s ).
 RNAPII synthesizes the precursor of
mRNA and some snRNAs.
 RNAPIII  synthesizes smaller RNAs
– 5srRNA, tRNA, snRNA.
Post transcriptional
modification
 A primary transcript is a linear copy
of a transcriptional unit, the segment
of DNA between initiator and
terminator sequences.
 The primary transcript of both tRNAs
and rRNAs are post transcriptionally
modified by cleavage of the original
transcripts by ribonucleases. tRNAs
are further modified.
r RNAs and t RNAs
 In eukaryotes single 45 s precursor
gives rise to 5.8s, 18s and 28s r
RNAs. 5s rRNA is produced from a
separate precursor molecule.
 30 s precursor in prokaryotes
produces 5s 16 s and 23 s r RNAs.
 Both pro and eukaryotic t RNAs are
made from longer precursors that
must be trimmed.
Messenger RNA
 Prokaryotic mRNA is generally
identical to its primary transcript,
whereas eukaryotic mRNA is
extensively modified after
transcription.
 tRNAs and rRNAs of both pro and
eukaryotes are modified after
transcription.
Post transcriptional
modification of mRNA
 Capping.
 Addition of poly A tail.
 Removal of introns.
 Methylation.
 RNA editing.
CAPPING
 The cap is 7 methyl guanosine tri
phosphate linked to the 5’ terminal of
the mRNA. The addition is catalyzed
by the enzyme guanylyl transferase.
The methylation of the terminal
guanine is catalyzed by the enzyme 7
methyl transferase S.adenosyl
methionine is the methyl donor.
Function of the CAP
 Facilitates the initiation of translation.
 Helps the recognition of mRNA by the
protein synthesizing machinery
(ribosome)
 Protects the mRNA from the action of
exonuclease.
Addition of poly A tail
 A chain of 40 – 200 adenine
nucleotides is attached to the 3’ end
of the primary transcript. This is
added by the enzyme poly A
polymerase.
 Most eukaryotic mRNAs have poly A
tail except histone mRNA.
 Function is to stabilize the mRNA.
After the mRNA enters the cytosol the
poly A tail is gradually shortened.
Intron removal
 From the primary transcript introns
are removed and the exons are
spliced together to form mature
mRNA.
 snRNAs are associated with proteins
to form snRNPs (small nuclear
ribonucleo proteins ) which facilitates
removal of introns and splicing of
exons.
 After intron removal mature mRNA
leave the nucleus and enter the
cytosol.
RNA editing
 Central dogma is DNA  RNA 
Protein. So change in DNA will be
reflected into RNA and into protein,
but sometimes the coding information
can be changed at the RNA level. This
is called RNA editing.
 example  apo B 100 and apo B 48,
both are synthesized from the same
mRNA by RNA editing.
Spliceosome
 SNRNP, associated with hnRNA at the
exon- intron junction form
spliceosome. It consists of hnRNA, 5
snRNAs ( U1, U2, U4, U5, U6) and
more than 50 proteins. collectively
they are also called ‘SNURP’.
 SNURPs position the RNA segments
for splicing, cut the exon- intron
junction, joins the exons to form a
continuous sequence after intron
removal.
Ribozyme
 They are RNA molecules with catalytic
activity. Several enzymatic actions have
been attributed to RNA.
 SnRNA intron removal and splicing.
 Peptidyl transferase  protein
synthesis.
 RNAse P modification of tRNA precursor.
 They have specificity and obey M.M.
kinetics.
Inhibition of RNA
Polymerase
 Actinomycin -D Elongation of RNA
chain is inhibited both in pro and
eukaryotes.
 Rifampicin inhibits bacterial RNAP.
 Acridine  acts in the same way as
actinomycin – D.
 3’ deoxy adenosine  causes
premature chain termination.
 α- aminitine  inhibits RNAPIII.
Promoter Region
(prokaryote)
 The promoter sequences are
clustered approximately 10 base pairs
and 35 base pairs upstream (-10 and
– 35 sequences) from the
transcription start site.
 5‘TATAAT3’ for the -10 bp sequence
( Prinbow box) and 5’TTGACA’ for –
35 sequence.
 All promoter sequences are
recognized by the some sigma
subunit of the RNAP.
Promoter (eukaryote)
 -25 to -30 bp upstream from the
transcription start site 5’TATAAAAG 3’
(TATA or hogness box).
 Sequence further upstream G.C box
and CAAT box.
 Enhancer and repressor sequence,
both upstream and downstream.
Lecture 5. Transcription.ppt
Lecture 5. Transcription.ppt

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Lecture 5. Transcription.ppt

  • 1. TRANSCRIPTION DR. Vishnu Kumar PROFESSOR AND HEAD, DEPT.OF BIOCHEMISTRY MPTMC, SIDDHARTH NAGAR COMPETENCY NUMBER BI 7.2
  • 2. LEARNING OBJECTIVES After completion of this lecture learner should be able to define/ Describe:  Synthesis of RNA from DNA template  The primary transcript  DNA dependent RNA polymerase  Steps of RNA synthesis  RNA Classes  Post Translational Modification
  • 3. Transcription Synthesis of RNA from DNA template. The sequence of ribonucleotides in RNA molecule is complementary to the DNTPs in one strand of DNA called the template strand or sense strand. The other strand is called the coding strand or anti sense strand because it is identical to the RNA except U for T.
  • 4.
  • 5. Direction & enzyme involved  The information in the template strand is read in 3’ 5’ direction & the RNA is synthesized in 5’  3’ direction.  Enzyme involved  DNA dependent RNA polymerase. The enzyme attaches itself at a specific on the DNA, the promoter site on the template strand. This is followed by initiation of RNA synthesis.
  • 6. The primary transcript  hnRNA generated by RNAP is promptly capped by 7-methyl guanosine tri phosphate, which will eventually appear in the mRNA. hnRNA contains both introns and exons.  The cap is necessary for protection of mRNA from the action of 5’ exonuclease, also for recognition of mRNA by the ribosome
  • 7. DNA dependent RNA polymerase  in E coli it exists as a core molecule having 5 subunits. 2 α, ββ‘ w. The core RNAP utilizes a protein factor called sigma factor.  Core enzyme + sigma factor = Holo enzyme.
  • 8.
  • 9. Steps o RNA synthesis  Initiation binding of holoenzyme to the template at the promoter site to form the initiation complex. This is the closed complex. By sigma factor there is unwinding of 2 DNA strands. open complex.  Binding is followed by a conformational change of the RNAP.
  • 10. Initiation Steps continued  First nucleotide usually a purine associates with the β subunit of the enzyme. This becomes the 5’ of the mRNA.  In the presence of four RNTPs the RNAP moves to the 2nd base in the template.  Sigma factor is released.
  • 11. Initiation  The enzyme polymerizes the ribonucleotides in a specific sequence that is dictated by template strand and interpreted by Watson and Crick’s base pairing rules. PPi is releases at every step.  A purine ribonucleotides is usually first polymerized into the RNA molecule.
  • 12.
  • 13. Elongation  Unlike DNAP, RNAP does not require a primer and does not have proof reading activity.  RNAP has unwindase activity which causes local unwinding of the DNA double helix.  As the RNAP pushes its way between the strands it creates a +ve super coiling ahead and - ve super coiling behind it. Which are released by DNA gyrases and topoisomerases
  • 14.
  • 15. Termination  Two types ‘ rho’ dependent and ‘ rho’ independent.  ‘rho’ dependent here termination is signaled by a sequence in the template strand of the DNA molecule (CA rich region) called ‘rut’ (rho utilization) a signal that is recognized by rho factor.  Rho protein has an ATP dependent helicase activity.
  • 16. Rho independent termination  The RNA transcript must be able to form a stable hairpin turn that slows down the progress of RNAP. The hairpin turn is complementary to a palindrome sequence  Following the hairpin turn the RNA transcript must have a string of ‘U’ s. the A=U bonding is weak which facilitates its separation from the DNA strand.
  • 17.
  • 18. Termination  After termination the core enzyme separates from the DNA template.  With the assistance of another sigma factor the core enzyme recognizes another promoter at which the synthesis of a new RNA molecule commences.
  • 19. Transcription of eukaryotic gene  Far more complicated process than that in prokaryotic gene.  In addition to RNAP recognizing the promoter region and initiating RNA synthesis , a number of transcription factors bind to distinct sites of DNA.  There are 3 classes of RNAP in the nucleus.
  • 20. RNAP – classes  RNAP1 synthesizes the 45S precursor of r RNA (5.8s, 18s, 28s ).  RNAPII synthesizes the precursor of mRNA and some snRNAs.  RNAPIII  synthesizes smaller RNAs – 5srRNA, tRNA, snRNA.
  • 21. Post transcriptional modification  A primary transcript is a linear copy of a transcriptional unit, the segment of DNA between initiator and terminator sequences.  The primary transcript of both tRNAs and rRNAs are post transcriptionally modified by cleavage of the original transcripts by ribonucleases. tRNAs are further modified.
  • 22. r RNAs and t RNAs  In eukaryotes single 45 s precursor gives rise to 5.8s, 18s and 28s r RNAs. 5s rRNA is produced from a separate precursor molecule.  30 s precursor in prokaryotes produces 5s 16 s and 23 s r RNAs.  Both pro and eukaryotic t RNAs are made from longer precursors that must be trimmed.
  • 23. Messenger RNA  Prokaryotic mRNA is generally identical to its primary transcript, whereas eukaryotic mRNA is extensively modified after transcription.  tRNAs and rRNAs of both pro and eukaryotes are modified after transcription.
  • 24. Post transcriptional modification of mRNA  Capping.  Addition of poly A tail.  Removal of introns.  Methylation.  RNA editing.
  • 25.
  • 26. CAPPING  The cap is 7 methyl guanosine tri phosphate linked to the 5’ terminal of the mRNA. The addition is catalyzed by the enzyme guanylyl transferase. The methylation of the terminal guanine is catalyzed by the enzyme 7 methyl transferase S.adenosyl methionine is the methyl donor.
  • 27. Function of the CAP  Facilitates the initiation of translation.  Helps the recognition of mRNA by the protein synthesizing machinery (ribosome)  Protects the mRNA from the action of exonuclease.
  • 28. Addition of poly A tail  A chain of 40 – 200 adenine nucleotides is attached to the 3’ end of the primary transcript. This is added by the enzyme poly A polymerase.  Most eukaryotic mRNAs have poly A tail except histone mRNA.  Function is to stabilize the mRNA. After the mRNA enters the cytosol the poly A tail is gradually shortened.
  • 29.
  • 30. Intron removal  From the primary transcript introns are removed and the exons are spliced together to form mature mRNA.  snRNAs are associated with proteins to form snRNPs (small nuclear ribonucleo proteins ) which facilitates removal of introns and splicing of exons.  After intron removal mature mRNA leave the nucleus and enter the cytosol.
  • 31.
  • 32. RNA editing  Central dogma is DNA  RNA  Protein. So change in DNA will be reflected into RNA and into protein, but sometimes the coding information can be changed at the RNA level. This is called RNA editing.  example  apo B 100 and apo B 48, both are synthesized from the same mRNA by RNA editing.
  • 33. Spliceosome  SNRNP, associated with hnRNA at the exon- intron junction form spliceosome. It consists of hnRNA, 5 snRNAs ( U1, U2, U4, U5, U6) and more than 50 proteins. collectively they are also called ‘SNURP’.  SNURPs position the RNA segments for splicing, cut the exon- intron junction, joins the exons to form a continuous sequence after intron removal.
  • 34. Ribozyme  They are RNA molecules with catalytic activity. Several enzymatic actions have been attributed to RNA.  SnRNA intron removal and splicing.  Peptidyl transferase  protein synthesis.  RNAse P modification of tRNA precursor.  They have specificity and obey M.M. kinetics.
  • 35. Inhibition of RNA Polymerase  Actinomycin -D Elongation of RNA chain is inhibited both in pro and eukaryotes.  Rifampicin inhibits bacterial RNAP.  Acridine  acts in the same way as actinomycin – D.  3’ deoxy adenosine  causes premature chain termination.  α- aminitine  inhibits RNAPIII.
  • 36. Promoter Region (prokaryote)  The promoter sequences are clustered approximately 10 base pairs and 35 base pairs upstream (-10 and – 35 sequences) from the transcription start site.  5‘TATAAT3’ for the -10 bp sequence ( Prinbow box) and 5’TTGACA’ for – 35 sequence.  All promoter sequences are recognized by the some sigma subunit of the RNAP.
  • 37.
  • 38. Promoter (eukaryote)  -25 to -30 bp upstream from the transcription start site 5’TATAAAAG 3’ (TATA or hogness box).  Sequence further upstream G.C box and CAAT box.  Enhancer and repressor sequence, both upstream and downstream.