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DNA Sequencing Scenario

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Presentation on theme: "DNA Sequencing Scenario"— Presentation transcript:

1 DNA Sequencing Scenario

2 DNA replication and chain termination
Adapted from Lehninger Principles of Biochemistry 4th Edition P T A C G ÖH OH dATP ddTTP No OH group = chain termination at T residue P H T Primer strand The 3´ hydroxyl (OH) group interacts with the phosphate group on the incoming nuclueotide to form a phosphodiester bond Template strand

3 Nucleosides & Nucleotides
Taken from: Nucleoside = a heterocyclic base (A, G, C, U or T) and a five carbon sugar (pentose) either ribose for RNA or deoxyribose for DNA Nucleotide = a heterocyclic base and a pentose sugar with one or more phosphate groups (mono-, di- or tri-phosphate). Nucleotides are the monomers of nucleic acids, with three or more bonding together in order to form a nucleic acid.

4 Nucleotide structure continued
Base H OH CH2 -O P O- Nucleoside tri-phosphate (NTP) With a ribose sugar (OH at C2 & C3) used to synthesise RNA. O Base H OH CH2 -O P O- Deoxynucleoside tri-phosphate (dNTP) With a deoxyribose sugar (OH at C3) used to synthesise DNA. O Base H CH2 -O P O- Dideoxynucleoside tri-phosphate (ddNTP) With a dideoxyribose sugar (no OH groups) used for the Sanger method (dideoxy) sequencing.

5 Nucleotides are joined together by phosphodiester bonds
phosphodiester bond Phosphodiester bonds require a hydroxyl group (OH) to be present on the 3´ carbon to react with a phosphate on in 5´ carbon of the sugar residue of the next nucleotide. If no 3´ hydroxyl group is available no further nucleotides can join the DNA strand and the chain terminates. This is how dideoxynucleotides prevent chain elongation – they lack a 3´ OH group on the sugar.

6 Outline of Fluorescent Dideoxy DNA Sequencing
Components of the reaction mix DNA template DNA primer DNA polymerase -Taq polymerase Mixture of deoxy (dNTPs) & fluorescently labelled dideoxy nucleotides (ddNTPs) 20 – 35 cycles Apply to a capillary gel & subject to electrophoresis Computer analysis – base calling The fragments are detected after excitation of the labelled ddNTPs by a laser Fluorescent peaks and bases are visualised and analysed

7 The sequencing reaction continued
Components in the reaction mix Taq polymerase PRIMER OH + dATP, dCTP, dGTP, dTTP, + ddATP, ddCTP, ddGTP, ddTTP TEMPLATE AGTCTATATC Termination products obtained Remember that the sequence obtained with be complementary to the template sequence! PRIMER T PRIMER TCAGAT PRIMER TCAGATA PRIMER TC PRIMER TCAGATAG PRIMER TCA TCAG PRIMER PRIMER TCAGA Therefore our new 5´  3´ complementary sequence to our original template sequence reads TCAGATAG.

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