Team:Caltech/Protocols/PABA HPLC assay
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+ | <div style="font-size:18pt;"> | ||
+ | <font face="verdana" style="color:#CC3300">para-Aminobenzoic Acid (pABA) HPLC Assay Protocol</font></div> | ||
+ | <br> | ||
+ | __TOC__ | ||
==Purpose== | ==Purpose== | ||
To test for para-aminobenzoic acid levels in ''E. coli'' overexpressing the pABA synthesis genes ''pabA'' and ''pabB''. | To test for para-aminobenzoic acid levels in ''E. coli'' overexpressing the pABA synthesis genes ''pabA'' and ''pabB''. | ||
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* Buffer B: 0.1% formic acid in MeOH | * Buffer B: 0.1% formic acid in MeOH | ||
* A high performance liquid chromatography machine. | * A high performance liquid chromatography machine. | ||
- | * Column | + | * HPLC Column: Eclipse XDB-C18 column, 5um particles, 4.6x150mm column, with attached guard column (all from Agilent) |
==Procedure== | ==Procedure== | ||
===Sample Prep=== | ===Sample Prep=== | ||
- | + | # Centrifuge the cell culture max speed, 10 minutes. | |
- | + | # Separate pellet from supernatant. | |
- | + | # Resuspend the pellet in 1mL 0.1M Tris-HCl buffer | |
- | + | # Sonicate the resuspended pellet for 1 minute, alternating between 0 and 12Hz. | |
- | + | # Filter sterilize the cell lysate and the supernatant. | |
- | + | # Load 500uL of each into the HPLC. | |
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===HPLC Method=== | ===HPLC Method=== | ||
- | + | # Injection volume was 20uL, column temperature was kept at 40°C. | |
+ | # Flush the lines individually with Buffer A and B for two minutes each, flush the column with 92% A, 8% B for 10 minutes. | ||
+ | # From the source: "The starting eluent was 92% A mixed with 8% B; the proportion of B was increased linearly to 50% in 7 min, then to 100% in 3 min. The mobile phase was then immediately adjusted to its initial composition and held for 4 min in order to re-equilibrate the column." | ||
+ | # We found the retention time of pABA to be 4.9-5.0 minutes, however the literature states the retention time as 6.0 minutes. | ||
- | + | [[Image:PABA Standard HPLC assay - 08-07-08.PNG|thumb|center|pABA eluting at 4.9-5.0 minutes for the standard curve.]] | |
- | + | ===Standard Curve=== | |
+ | 1. Run 1:3 dilutions starting from 10ug/ml pABA in wild type bacterial lysate using the same protocol to generate a linear standard (see below). | ||
- | + | [[Image:08-07-08_pABA_Standard_Curve_plot.jpg | thumb|center |pABA HPLC standard curve with 1:3 dilutions starting from 10ug/ml pABA. The integral of the peak is plotted against the known pABA amount.]] | |
- | === | + | ===Sources=== |
- | + | Guo-Fang Zhang, Kjell A. Mortier, Sergei Storozhenko, Jet Van De Steene, Dominique Van Der Straeten, Willy E. Lambert. ''Free and total para-aminobenzoic acid analysis in plants with high-performance liquid chromatography/tandem mass spectrometry.'' '''Rapid Communications in Mass Spectrometry''': Volume 19, Issue 8 , Pages 963 - 969, 2005. | |
- | == | + | ===Contacts=== |
- | + | [[User:vhsiao|Victoria Hsiao]] | |
+ | }} |
Latest revision as of 20:55, 15 October 2008
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para-Aminobenzoic Acid (pABA) HPLC Assay Protocol
PurposeTo test for para-aminobenzoic acid levels in E. coli overexpressing the pABA synthesis genes pabA and pabB. Materials
ProcedureSample Prep
HPLC Method
Standard Curve1. Run 1:3 dilutions starting from 10ug/ml pABA in wild type bacterial lysate using the same protocol to generate a linear standard (see below). SourcesGuo-Fang Zhang, Kjell A. Mortier, Sergei Storozhenko, Jet Van De Steene, Dominique Van Der Straeten, Willy E. Lambert. Free and total para-aminobenzoic acid analysis in plants with high-performance liquid chromatography/tandem mass spectrometry. Rapid Communications in Mass Spectrometry: Volume 19, Issue 8 , Pages 963 - 969, 2005. Contacts |