The Mechanism of Transcription in Bacteria Chapter 6
RNA Polymerase Structure 1969 SDS-PAGE of E.coli RNA polymerase - 2 very large subunits are β (150 kD) and β’ (160 kD) –Sigma (σ) at 70 kD –Alpha (α) at 40 kD – 2 copies present in holoenzyme –Omega (ω) at 10 kD
Specificity factor Holoenzyme and Core enzyme Core enzyme transcribes both DNA strands Without σ-subunit the core enzyme has basic transcribing ability but lacks specificity
Promoters Presence of the σ-subunit permitted recognition of authentic RNA polymerase binding sites Polymerase binding sites are called promoters Transcription that begins at promoters is specific - directed by the σ-subunit
Binding of RNA Polymerase to Promoters Experiment measures binding of DNA to enzyme using nitrocellulose filters –Holoenzyme binds filters tightly –Core enzyme binding is more transient
Temperature and RNA Polymerase Binding As temperature is lowered, the binding of RNA polymerase to DNA decreases dramatically Higher temperature promotes DNA melting
Promoter Sequence
Core Promoter Elements There is a region common to bacterial promoters described as 6-7 bp centered about 10 bp upstream of the start of transcription = -10 box Another short sequence centered 35 bp upstream is known as the = -35 box Comparison of thousands of promoters has produced a consensus sequence for each of these boxes
Promoter Structure Consensus sequences: –-10 box sequence approximates TAtAaT –-35 box sequence approximates TTGACa Mutations that weaken promoter binding: –Down mutations –Increase deviation from the consensus sequence Mutations that strengthen promoter binding: –Up mutations –Decrease deviation from the consensus sequence
rrnB promoter in E.coli UP promoter element stimulating transcription by a factor of 30 UP is associated with 3 “Fis” sites.
Polymerase/Promoter Binding Holoenzyme binds DNA loosely Complex loosely bound at promoter = closed promoter complex - dsDNA in closed form Holoenzyme melts DNA at promoter forming open promoter complex - polymerase tightly bound
Initiation and Elongation Transcription
Stages of Transcription Initiation Formation of a closed promoter complex Conversion of the closed promoter complex to an open promoter complex Polymerizing the early nucleotides – polymerase at the promoter Promoter clearance – transcript becomes long enough to form a stable hybrid with template
Functions of σ Gene selection for transcription by σ causes tight binding between RNA polymerase and promoters Tight binding depends on local melting of DNA that permits open promoter complex Dissociation of σ from core after sponsoring polymerase-promoter binding
Reuse of σ During initiation σ can be recycled for additional use in a process called the σ cycle Core enzyme can release σ which then associates with another core enzyme
σ May Not Dissociate from Core During Elongation The σ -factor changes its relationship to the core polymerase during elongation It may not dissociate from the core May actually shift position and become more loosely bound to core
Local DNA Melting at the Promoter It was calculated that each polymerase caused a separation of about 10 bp In another experiment, the length of the melted region was found to be 12 bp Size of the DNA transcription bubble in complexes where transcription was active – bp
Structure and Function of σ Genes encoding a variety of σ -factors have been cloned and sequenced There are striking similarities in amino acid sequence clustered in 4 regions Conservation of sequence in these regions suggests important function All of the 4 sequences are involved in binding to core and DNA
Homologous Regions in Bacterial σ Factors
Region 1 Role of region 1 appears to be in preventing σ from binding to DNA by itself This is important as σ binding to promoters could inhibit holoenzyme binding and thereby inhibit transcription
Region 2 Most highly conserved of the four Four subregions – 2.1 to recognizes the promoter’s -10 box The 2.4 region appears to be α-helix
Region 3 and 4 Region 3 is involved in both core and DNA binding Region 4 is divided into 2 subregions –This region seems to have a key role in promoter recognition –Subregion 4.2 contains a helix-turn-helix DNA- binding domain and appears to govern binding to the -35 box of the promoter
Role of α-Subunit in UP Element Recognition RNA polymerase binds to a core promoter via its σ- factor - no help from C- terminal domain of α- subunit Binds to a promoter with an UP element using σ plus the α -subunit C- terminal domains Results in very strong interaction between polymerase and promoter This produces a high level of transcription
Elongation After transcription initiation is accomplished, core polymerase continues to elongate the RNA Nucleotides are added sequentially, one after another in the process of elongation
Function of the Core Polymerase Core polymerase contains the RNA synthesizing machinery Phosphodiester bond formation involves the β- and β’-subunits β- and β’-subunits also participate in DNA binding Assembly of the core polymerase is a major role of the α-subunit
Topology of Elongation Elongation of transcription involves polymerization of nucleotides as the RNA polymerase travels along the template DNA Polymerase maintains a short melted region of template DNA DNA must unwind ahead of the advancing polymerase and close up behind it Strain introduced into the template DNA is relaxed by topoisomerases
Termination of transcription There are 2 main types of terminators –Intrinsic terminators function with the RNA polymerase by itself without help from other proteins –Other type depends on auxiliary factor called - ρ - dependent terminators
Chain Termination Two types of termination mechanisms: intrinsic termination- controlled by specific sequences, termination sites Termination sites characterized by two inverted repeats
Rho-Independent Termination The repeat at right is symmetrical around its center shown with a dot A transcript of this sequence is self- complementary –Bases can pair up to form a hairpin –Inverted Repeats and Hairpins
Model of Intrinsic Termination Bacterial terminators act by: Base-pairing of something to the transcript to destabilize RNA-DNA hybrid –Causes hairpin to form Causing the transcription to pause –Causes a string of U’s to be incorporated just downstream of hairpin
Mechanism of ρ dependent termination Binding to the growing transcript - ρ follows the RNA polymerase Catches the polymerase as it pauses at the hairpin Releases transcript from the DNA-polymerase complex by unwinding the RNA-DNA hybrid
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