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What is 4Q7Q?
In 2000, the protein structure initiative (PSI) began with the goal of finding the three dimensional structure of as many proteins as possible. In 2010, however, funding for the PSI was terminated. Nevertheless, millions of protein structures were found, and many structures were uncharacterized. One of these uncharacterized proteins found in Chitinophaga pinesis. Its molecular weight is 87.1 kDa. Through structural and sequential analysis on BLAST, PFam, Dali, and ProMol, 4Q7Q is believed to be a lipase.
Sequential analysis of 4Q7Q
BLAST-Sequence homology between 4Q7Q was tested through BLAST; the top hit for 4Q7Q was 4M8K, a GDSL-like lipase. 4Q7Q and 4M8k share a 36% sequence homology, but a low E-value, indicating it is a significant match.
PFam-Results from PFam sequence mapping also indicated that 4Q7Q shares sequence homology with other GDSL-like lipases.
Snapgene-Snapgene was able to reveal the molecular mass of 4Q7Q, later used as a reference when its purified form was run on an SDS-page gel. Snapgene also provided information about tags used to insert its gene into the plasmid used for transformation in DH5α and BL21 E. coli cells.
Structural analysis of 4Q7Q
Dali-Top hits from Dali indicated that 4Q7Q shares structural homology with putative lipases.
ProMol-Through ProMol, a possible catalytic triad for 4Q7Q (Ser164, Asp193, His196) was found due to catalytic triad alignment with 1BRW. 4Q7Q and 1BRW catalytic triad alignment yielded a RMS value of 2.049, and a full structural homology with an RMS value of 4.852.
Enzymatic Assay of 4Q7Q
Reasoning-Results obtained in silico strongly suggested that 4Q7Q was most likely to be hydrolase, and specifically a lipase. Thus, a lipase assay was run on 4Q7Q to confirm its enzymatic function. The lipase assay conducted was done through spectrophotometric methods. Purified 4Q7Q was mixed in solution with P-nitrophenyl butyrate. When nitrophenyl butyrate undergoes hydrolysis, its products are p-nitrophenol and butyrate. P-nitrophenol’s color becomes yellow when this reaction happens in solution.Thus, when a lipase catalyzes the hydrolysis of P-nitrophenol butyrate, a color change in solution will occur. A colorimeter was set at 430nm to detect light in the “yellow” range and thereby measure the change in color occuring when 4Q7Q catalyzed the hydrolysis reaction.
4.2 Results
Conclusion-Due to 4Q7Q’s low concentration found on the SDS-page gel, 4Q7Q to pNPB ratio in solution was 10:1. A logarithmic-curve was present during the lipase assay conducted on 4Q7Q, indicating it successfully catalyzed the hydrolysis of a lipid.
Future directions
Cloning-To confirm the suspected catalytic triad of 4Q7Q, site directed mutagenesis of 4Q7Qs catalytic triad was performed through PCR. Substitutions of residues were completed as followed: Ser164Ala, Asp193Ala, His196Ala. Following a successful cloning, a p-NPB lipase assay will be performed to see whether the new mutations on 4Q7Q deterred catalysis of the hydrolysis reaction of p-NPB.
Enzyme Kinetics of 4Q7Q=Further data of enzyme activity of 4Q7Q using our lipase assay at different concentrations of p-NPB can be performed to create a Lineweaver-Burk plot.
Optimization of enzymatic activity-Conditions for optimized enzyme activity can be tested by doing pH and temperature iterations of the p-NPB assay.
