Sandbox2O14
From Proteopedia
(Difference between revisions)
| Line 6: | Line 6: | ||
<StructureSection load='2o14-assembly1.cif.gz' size='400' side='right' caption='3D Representation of 2O14’s structure' scene=''> | <StructureSection load='2o14-assembly1.cif.gz' size='400' side='right' caption='3D Representation of 2O14’s structure' scene=''> | ||
| + | |||
| + | == Overview == | ||
| + | |||
| + | 2O14 exists as monomeric protein complex. Using SPRITE and Chimera revealed one chain that is very long and does not replicate the amino acid chain. This was further confirmed by looking at the X-ray structure of protein 2O14 and it is stating that there is only one unique protein chain. The chain is 366 residues long and the entire complex has a molecular weight of approximately 41.79kDa. | ||
| + | |||
| + | 2O14 proteins originated from the bacterial species bacillus subtills. InterPro results showed how almost all similar enzymes came from bacterial species like the bacillus subtills. It was also found to not be in any viruses, but a small fraction could be found in archaea, eukaryote and other small organisms. | ||
| + | |||
| + | == Family and Superfamily == | ||
| + | The data found showed that 2O14 is like a Rhamnogalacturan_acetylesterase that falls under the SGNH Hydrolase protein super family. Using a SPRITE analysis, we found that the lower RMSD values match was with 1bwp_c01 a Platelet Act Factor with a value of 0.60 and matched with aspargine, aspartic acid and histidine residues, for the right-hand superposition. Looking at the left-hand superposition, the lowest RMSD value was 0.62 with 1xny_c01, propionyl-COA carboxylase complex B, and its matching residues were 1 alanine and two glycine groups. | ||
| + | |||
| + | Using the data gotten from the DALI software, it was found that protein 1k7c or rhamnogalacturonan acetylesterase had the most matching amino acids, 98, creating a z score pf 25.1 create a 25.1% match to protein 2O14. Furthermore, using DALI stacked Pfam data graphics showed that protein 2O14 was a potential member of GDSL-like Lipase/Acylhyydrolase family. This would agree with data gather from InterPro that stated that 2O14 was most likely resembling a rhamnogalacturonan acetylesterase. | ||
| + | |||
| + | When using BLAST, the group was able to not only look at 2O14 amino acid sequence but also its taxonomy which showed that the protein was seen in the Bacillota superfamily which is a phylum of bacteria that have gram positive cell walls. Furthermore, for this phylum of bacteria it is very common for them to contain multiple hydrolases including SGNN hydrolases like 2O14. | ||
| + | |||
| + | |||
| + | == Sequence Analysis == | ||
| + | |||
| + | Analysis of the primary structure of 2O14 began in SPRITE. Right-handed superposition analysis related two possible enzymes to 2O14, 1BWP and 1PP4. RMSD values for 1BWP and 1PP4 were 0.92 and 0.93 respectively and both proteins matched five residues with 2O14. 1BWP is defined as “Platelet-activating factor acetyl hydrolase,” and 1PP4 is defined as “Rhamnogalacturonan acetyl esterase.” | ||
| + | The primary structure of 2O14 exhibits its active site through the specific residues of Ser171, Gly209, Asn241, Asp339, and His342. This active site spans residues 170 to 350 with this region defined as “Rhamnogalacturonan acetyl esterase like” and falling into the SGNH hydrolase superfamily through BLAST analysis of the primary structure. | ||
| + | Analysis of the primary sequence alone showed promising signs of 2O14 acting as a hydrolase due to its relation to RGAE through its active site and the SGNH hydrolase superfamily. | ||
| + | |||
| + | == Structural Analysis == | ||
| + | |||
| + | 2O14 contains several similarities secondary structures to proteins 1K7C and 1PP4. 2O14 exhibits a GDSL 2 sequence motif, a variant of the GDSL motif exhibited in both 1K7C and 1PP4. Structural analysis using the Dali software showed both proteins superimposed over 2O14 with z-scores of 25.1 and 24.8 respectively. These two proteins are defined as rhamnogalacturonan acetyl esterases. | ||
| + | After obtaining data from SPRITE, 2O14 was superimposed onto 1PP4 giving an angstroms difference of 0.736Å. This mostly came in the alpha helix region both proteins where the proposed active site is located. Through all analyses, the beta sheet region of 2O14 had no hits relating to its structure or sequence. | ||
| + | Analysis of the structure further emphasized the similarities to RGAE and the proposed function of 2O14 being a hydrolase of some kind, either a lipase or esterase. | ||
| + | |||
| + | == Substrates == | ||
| + | |||
| + | SwissDock analysis was done on specific substrates including 4-Nitrophenyl alpha-glucoside, 2-acetamido-2-deoxy-beta-D-glucopyranose, and p-nitrophenyl phosphate. Both PNPG and GlcNac exhibited high binding affinities to 2O14. This would be due 2O14’s proposed enzymatic function. | ||
| + | |||
| + | == Theoretical Functionality and Proposed Bodily Purpose == | ||
| + | |||
| + | During our research and experiments the group had used SwissDock to potentially bind to protein 2O14. The determined smile code for the protein was C1=CC(=CC=C1[N+](=O)[O-])O[C@@H]2[C@@H]([C@H]([C@@H]([C@H](O2)CO)O)O)O, and found relatively low calculated affinity values ranging from -6.133 to -3.387. The SwissDock predicted four binding sites it believed molecules could interact with the protein at. One inside the protein itself as shown in Figure 1. Other spaces that were seen to have good binding affinity were outside of the protein embedded in the side, Figure 2, And then finally on the side in Figure 3. The two more likely cases of binding are figures 2 and 3, however, figure 1 had the lowest binding affinity. | ||
| + | |||
| + | Each of the binding affinities correlated with some kind of saccharide, each saccharide was found to interact with acetyl esterases. Furthermore, all the prior data had shown that protein 2O14 was most like an acetyl esterase being most closely related to Rhamnogalacturan acetylesterase, the group decided to experiment on the protein using PNPP to see whether their protein interacted with it. | ||
| + | |||
| + | After performing all the necessary steps to extract the protein, it was found that most of the protein came out in the first elution, elution 1. Then using UV-Vis, 10µL of protein solution was added to a cuvette with a 10:1 ratio of PNPP and PNPP buffer solution. This showed an instantly yellow solution, so it was believed that protein was in the elution. We did the same test again with elution 2, to confirm that the protein was in elution 1, and had similar results. The group then attempted to adjust the pH to be more like dirt and soil pH and got completely opposite results, where the absorbance of the first two tests was around 0.95 and the pH test was around 0.09. With these completely opposite results, it was unclear if elution 1 had the protein. Figures 4, 5, and 6 show the explained experiments above in order. | ||
| + | |||
| + | == Figure 4 == | ||
| + | Protein test using 10µL of protein from elution and 30mg of PNPP and 3mL of PNPP solution. Measuring absorbance at 405M. | ||
Revision as of 23:37, 27 April 2025
2O14 Structure and Proposed Functionality
(NOTE TO ALL EDITORS: This page is part of a final project for a biochemistry lab at Elizabethtown College. Please do not edit this.)
2O14 is a monomeric protein complex that originates from the bacterial species Bacillus subtilis and has a mass of 41.79 kDa. Using InterPro this protein was assumed to be like Rhamnogalacturan acetylesterase, which falls under the SGNH Hydrolase Superfamily with structural and sequential similarities to lipases, esterases, along with similar functional domains to galactose-binding. With the research performed with current protein databases available, the evidence suggests that this protein removes acetyl groups from the backbone proteins by hydrolyzing the acetyl esters. It accomplishes this most likely through the catalytic triad of serine-histidine-aspartic acid.
| |||||||||||
