Revision as of 14:47, 30 September 2013

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- Pre-processing: Signal diffusion
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What about those hydrolases ?

Colisweeper depends largely on processing of molecular signals and generation of visible and distinguishable color outputs used as logic to play the game. Next to our P_LuxR promoter mutations, which detect ranges of OHHL concentrations, we make use of a reporter system which gives colorimetric responses only to be triggered by the player. As our reporter system, we rely on a set of orthogonal hydrolase enzymes that are native to Escherichia coli. These hydrolases include the Citrobacter alkaline phospohatase, the Bacillus subtilis β-glucuronidase and the Escherichia coli acetylesterase, β-N-Acetylglucosaminidase and β-galactosidase. In order to prevent background expression of these native hydrolases in Escherchia coli, we use a triple knockout strain that has three hydrolase genes knocked out: gusA (β-glucuronidase), aes (acetylesterase) and nagZ (β-N-acetylglucosaminidase). Addition of a multi-substrate mix by the player leads to an enzyme-susbtrate reaction which specifically cleaves the chromogenic substrates, thereby producing a visible color output.

β-Glucuronidase (gusA)

gusA encodes β-Glucuronidase, an intracellular enzyme that catalyzes the hydrolysis of β-D-glucuronides. This is a 68 kDa tetrameric enzyme with the E.coli homolog name as uidA. It is commonly used as a reporter system for various experimental measurements. See more details in the part registry for gusA [http://parts.igem.org/Part:BBa_K1216000 click here]

Alkaline phosphatase (phoA)

The alkaline phosphatase is a periplasmic homodimeric hydrolase. Each monomer contains 429 amino acids. This monomer is a dimer of 51 kDa. See more details in the part registry for phoA [http://parts.igem.org/Part:BBa_K1216001 click here]

Acetyl esterase (aes)

The Escherichia coli acetyl esterase is encoded by the aes gene and has been identified as a member of the hormone-sensitive lipase family (1). Acetyl esterase interferes with the expression of the maltose system by counteracting maltose sensitivity (5). This cytosolic enzyme is a 36 kDa monomer and catalyzes hydrolysis of substrates with an acyl chain length of less than 8 (1). It is composed of 319 amino acid residues (2) and its catalytic triad is composed of Ser165, Asp262 and His292 (3). Various substrates can used for chromogenic enzyme assays, e.g. p-nitrophenyl butanoate (4), p-nitrophenyl acetate (5) and p-nitrophenyl butyrate (6). Kinetic constants for Aes are K_m 17 +/- 4.1 x 10^-5 M and K_cat 29 +/- 3.0 s^-1 when using p-nitrophenyl butyrate as a substrate (6).
In Colisweeper, 5-Bromo-6-Chloro-3-indoxyl butyrate is used in the multi-mix substrate. After hydrolysis of this substrate, an indigo analog precipitates, which absorbs at 565 nm (visible as magenta color).
This enzyme's coding region has been added to the registry by our team as [http://parts.igem.org/Part:BBa_K1216002 K1216002]. We used this part in our final circuit and have made this our favorite part.

β-N-Acetylglucosaminidase (nagZ)

The β-N-Acetylglucosaminidase enzyme from Escherichia Coli encoded by the nagZ gene, is a cytoplasmatic hydrolase which is involved in the cell wall recycling pathway. This enzyme is also of therapeutic interest as it is involved in the hyperproduction of the AmpC β-lactamase in gram-negative bacteria [http://www.cazypedia.org/index.php/Glycoside_Hydrolase_Family_3 1]. See more details in the part registry for nagZ [http://parts.igem.org/Part:BBa_K1216003 click here]

β-Galactosidase (LacZ)

References

(1) Kanaya S, Koyanagi T, Kanaya E, Biochem. J., 332, 75-80 (1998).
(2) Blattner FR, Plunkett III G, Bloch CA, Perna NT, Burna V, Riley M, Collado-Vides J, Glasner JD, Rode CK, Mayhew GF, Gregor J, Davis NW, Kirkpatrick HA, Goeden MA, Rose DJ, Mau B, Shao Y, Science, 277, 1453-1461(1997).
(3) Haruki M, Oohashi Y, Mizuguchi S, Matsuo Y, Morikawa M, Kanaya S, FEBS Lett., 454, 262-266 (1999).
(4) Farias T, Mandrich L, Rossi M, Manco G, Protein Pept. Lett., 14, 65-69 (2007).
(5) Peist R, Koch A, Bolek P, Sewitz S, Kolbus T, Boos J, J. Bacteriol., 179, 7679-7686 (1997).
(6) Kobayashi R, Hirano N, Kanaya S, Haruki M, Biosci. Biotechnol. Biochem., 76 (11), 2082-2088 (2012).

We thank our sponsors:

@@ Line 16: / Line 16: @@
 <h1>Acetyl esterase (''aes'')</h1>
-<p>
+<p align="justify">The ''Escherichia coli'' acetyl esterase is encoded by the ''aes'' gene and has been identified as a member of the hormone-sensitive lipase family (1). Acetyl esterase interferes with the expression of the maltose system by counteracting maltose sensitivity (5). This cytosolic enzyme is a 36 kDa monomer and catalyzes hydrolysis of substrates with an acyl chain length of less than 8 (1). It is composed of 319 amino acid residues (2) and its catalytic triad is composed of Ser165, Asp262 and His292 (3). Various substrates can used for chromogenic enzyme assays, e.g. p-nitrophenyl butanoate (4), p-nitrophenyl acetate (5) and p-nitrophenyl butyrate (6). Kinetic constants for Aes are K<sub>m</sub> 17 +/- 4.1 x 10<sup>-5</sup> M and K<sub>cat</sub> 29 +/- 3.0 s<sup>-1</sup> when using p-nitrophenyl butyrate as a substrate (6).
-This enzyme is a 36 kDa monomer that is present in the cytosol. It catalyses hydrolysis of p-nitrophenyl esters of fatty acids. The enzyme is involved in the regulation of the maltose operon. See more details in the part registry for ''aes'' [http://parts.igem.org/Part:BBa_K1216002 click here] </p>
+<br>
+In Colisweeper, 5-Bromo-6-Chloro-3-indoxyl butyrate is used in the multi-mix substrate. After hydrolysis of this substrate, an indigo analog precipitates, which absorbs at 565 nm (visible as magenta color).
+<br>
+This enzyme's coding region has been added to the registry by our team as [http://parts.igem.org/Part:BBa_K1216002 K1216002]. We used this part in our final circuit and have made this our favorite part. </p>
@@ Line 30: / Line 33: @@
 <h1>References</h1>
+(1) Kanaya S, Koyanagi T, Kanaya E, Biochem. J., 332, 75-80 (1998).<br>
+(2) Blattner FR, Plunkett III G, Bloch CA, Perna NT, Burna V, Riley M, Collado-Vides J, Glasner JD, Rode CK, Mayhew GF, Gregor J, Davis NW, Kirkpatrick HA, Goeden MA, Rose DJ, Mau B, Shao Y, Science, 277, 1453-1461(1997).<br>
+(3) Haruki M, Oohashi Y, Mizuguchi S, Matsuo Y, Morikawa M, Kanaya S, FEBS Lett., 454, 262-266 (1999).<br>
+(4) Farias T, Mandrich L, Rossi M, Manco G, Protein Pept. Lett., 14, 65-69 (2007).<br>
+(5) Peist R, Koch A, Bolek P, Sewitz S, Kolbus T, Boos J, J. Bacteriol., 179, 7679-7686 (1997).<br>
+(6) Kobayashi R, Hirano N, Kanaya S, Haruki M, Biosci. Biotechnol. Biochem., 76 (11), 2082-2088 (2012).<br>
 <br clear="all"/>
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