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Assignment To find the mutation being introduced into the p53 protein if the primer sequence provided was used to run the PCR (note: the primer might be either a forward or a reverse sequence) PRIMER SEQUENCE STEP 1: Obtain the p53 nucleotide sequence from PUBMED database. Go to the PUBMED database and select ‘Nucleotide’ in the dropdown menu Type in p53 in the search box and click search. Select Homo Sapiens in the ‘Results by taxon’ section. Select the first p53 mRNA sequence shown (Note: this is a complete coding sequence for the p53 protein), 2,451 bp linear mRNA, Accession: AB082923.1, GI: 23491728 At the very end of the page, you will see the nucleotide sequence of the p53 protein. Immediately above the sequence, there is the amino acid sequence under the subheading ‘CDS’. Click CDS to highlight the coding region in the nucleotide sequence. Now copy the nucleotide sequence into the space below and highlight the CDS region in red: STEP 2: Compare and find out which region your particular primer binds to in the p53 coding sequence. Using google, search for ‘nucleotide blast’ – an NCBI sequence alignment program and open the following page. Copy and paste your primer sequence in the QUERY box and your p53 nucleotide sequence in the SUBJECT box. Click on BLAST. The colourful box shows a visual representation of your results while the exact nucleotide matches are shown below. The query sequence (1-29 nucleotides in length) matched exactly to the subject sequence from its nucleotide sequence starting from 194-222. Now go back to your nucleotide sequence and highlight in yellow, the corresponding region (194-222). NOTE: There will be a mismatch of one nucleotide (which is your mutation). Also, the reverse primers will map in the 3’ to 5’ direction. STEP 3: Find out which amino acid is being mutated and what the mutation is. Copy your CDS (coding sequence highlighted in red) from the nucleotide sequence below. A codon is a group of three nucleotides coding for a single amino acid. Please refer to the codon table provided below to know the composition of each amino acid. As you will notice, ATG is a start codon (first codon of your sequence in red) and TGA is a stop codon (last codon of your sequence in red). Amino acid Ala/A Codons GCT, GCC, GCA, GCG CODON TABLE Compressed Amino acid GCN Leu/L Codons TTA, TTG, CTT, CTC, CTA, CTG YTR, CTN AAR Arg/R CGT, CGC, CGA, CGG, AGA, AGG CGN, MGR Lys/K AAA, AAG Asn/N Asp/D Cys/C AAT, AAC GAT, GAC TGT, TGC AAY GAY TGY Met/M Phe/F Pro/P Gln/Q CAA, CAG CAR Ser/S ATG TTT, TTC CCT, CCC, CCA, CCG TCT, TCC, TCA, TCG, AGT, AGC Glu/E GAA, GAG GAR Thr/T Gly/G GGT, GGC, GGA, GGG CAT, CAC ATT, ATC, ATA GGN Trp/W CAY ATH Tyr/Y Val/V His/H Ile/I START ATG (adapted from WIKIPEDIA) STOP Compressed TTY CCN TCN, AGY ACT, ACC, ACA, ACG TGG ACN TAT, TAC GTT, GTC, GTA, GTG TAA, TGA, TAG TAY GTN TAR, TRA Next, split your above sequence into groups of three (i.e. into each codon) as shown below. 1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 Now, copy and paste below the highlighted primer region and pick out the mutation site and fill it in the box given below. Primer sequence in codons: is the codon being mutated. Using your codon table, identify which amino acid the above codon (in the box) codes for and write it below. codes for the following amino acid ___________________________ . From your primer sequence, identify the nucleotide that has been mutated. Has been mutated to which means that the amino acid has been mutated to . Please fill out the following sentence as your result from this exercise: In the ______ amino acid position, the codon ____________ has been mutated to __________ which means that the amino acid ________________________ has been changed to _________________________ . This can be represented using the notation ______________________ . EXERCISE A protein’s secondary structures may be visualized in 3D using various softwares like DeepView. These structures are generated using different techniques, for e.g. x-ray crystallography and published in various journals. All these structures are also available in databases like RCSB protein data bank (see below). In this exercise, we shall look into the p53 protein structure and observe the mutations being introduced in this project. I have previously downloaded the p53 homotetramer structure, PDB ID: A2HI. Open this structure using the DeepView software. We can see the various control and visualization panels below: We can un-highlight a single p53 protein using the control panel (right). Now, we can highlight a particular mutation, for e.g. R248G which is a change from Arginine to Glycine at the 248th position, using the control panel. In this structure we can observe Arginine at the 248th position. In the PCR we did yesterday, one set of primers introduced a change in this particular Arginine and changed it into a Glycine. Likewise, you may also study how this would affect various changes like DNA binding effects (if the mutation is in the DBD domain), electrostatic potentials, creation and deletion of different types of bonds, etc using this software. A pdf manual for this software is available for your perusal in your downtime. You may also find other p53 structures with other mutations in the RCSB database. Some examples are below: 1) V143A - http://www.rcsb.org/pdb/explore.do?structureId=2j1w PDB ID code 2J1W 2) R248G - http://www.nature.com/onc/journal/v26/n15/fig_tab/1210291f1.html#figure-title PDB ID code 2AHI 3) R175H - http://www.nature.com/onc/journal/v26/n15/fig_tab/1210291f1.html#figure-title PDB ID code 2AHI