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Results

Abstract

Itaconic Acid

SDS-Page

The expression of cadA has been visualized via SDS-PAGE. Positive clones were grown at 37° celsius until an OD of 0,7. Afterwards the cells were induced utilizing 20µl of 1M IPTG for 12h at 28° celsius. Finally the cells were lysated via ultrasonic cell disruption.

cadA Assay

The decarboxylic activity of cadA was shown via a pH indicator assay. As a byproduct of the catalytic conversion of cis-aconitate to itaconic acid carbon dioxide is released into the assay mixture. Here it forms carbonic acid and thereby lowers the pH value of the mixture. This is visualized through the indicator bromothymol blue (BTB) which changes its configuration state depending on the surrounding pH-Value (pH 6.0 - 7.6). That change of configuration can be shown via a photometric analysis in a TECAN® Infinite 200 PRO microplate reader. The resulting data sheets are then put into a plotting script written in R and exported as a ggplot. The assay was performed as following:
First Na₂HPO₄ was adjusted to a pH of 7.0 to function as a buffer. The final concentration of Na₂HPO₄ was 5mM. The assay system contained 10% (v/v) indicator stock (BTB) and 20 ul were added per well. As a negative control a purified TES protein fraction from disrupted BL21 cells was used. In a range from 0mM to 1mM (0,2mM steps; total of 6 reactions) cis-aconitate (substrate), dissolved in Na₂HPO₄-buffer solution was added per well to enable the enzymatic conversion. To put the turnover into relation with the maximum turnover we added extra rows that contained equal amounts of substrate and product (itaconic acid). Finally a row containing just itaconic acid was put at the bottom to be able to use the resulting values as a blank for the assay. All samples were prepared on ice. The 96 well microplate was loaded as depicted in the picture below:

The assay was run for 200 kinetic cycles, each 30 secs long and with 25 photo pulses per cycle. The reader was heated to the appropriate temperature of 37° celsius. Absorbance was measured at the absorption maximum of BTB which in this case is 620nm.

• The 'p' curve shows the absolute conversion of educt to product (product curve).
• The 'ca' curve shows the enzymatic activity of cadA. The activity explains the steady rise of the curve which comes from the acidification of the assay mixture in those wells. Because of the conversion from cis-aconitate to itaconic acid and the byproduct carbon dioxide (which forms bicarbonate acid) and lowers the pH
• The 'k' curve shows the negative control containing TES protein fraction without cadA.

The sudden drop of the 'p' curve in the beginning of the measurement could be explained through various reasons. One could be that the bubbles that formed in the wells when adding the chemicals could interfere with the light. Also the different substances were added on ice so when the plate was put in the heated reader water in the air might have condensated at the bottom of the wells and hinder the light beam. The resulting vibrations of shutting doors too harshly might also interfere with the plate moving mechanism inside the reader and cause malfunctioning.

The code utilized to render the plots is embedded at the bottom of the page.

Ethylene Glycol

Xylitol

SDS-Page

The expression of GRE3 has been visualized via SDS-PAGE. Positive clones were grown at 37° celsius until an OD of 0,5. Afterwards the cells were induced utilizing 20µl of 1M IPTG for 10h at 28° celsius. Finally the cells were lysated with heat and the suspension was put on the PAGE.

GRE3 assay

To prove the enzymatic activity of the aldose reductase GRE3 in dependance of NADPH we designed an applicable assay as following. We used a spectral analysis with a wavelength of 340nm to make the conversion from NADPH to NADP⁺ observable. A drop in the curve of the absorption spectrum therefore shows that NADPH is being converted to NADP+ i.e. the enzyme works. Spectral analysis was performed with a TECAN® Infinite 200 PRO microplate reader. The resulting data sheets are then put into a plotting script written in R and exported as a ggplot.

The assay was performed as described below:

First Na₂HPO₄ was adjusted to a pH of 7.0 to function as a buffer. The final concentration of Na₂HPO₄ was 0,1M. The assay system contained 0,1mM NADPH and 8 µl were added per well. As a possible blank wells with just NADPH (8 µl to 192 µl of buffer solution) were provided. In addition we added blanks containing just xylitol (0,1M) as well as one containing just NADP+ (0,1mM). The negative control contained a purified TES protein fraction from disrupted BL21 cells. The assay mixture included 154 µl buffer solution, 8 µl xylose, 8 µl NAPDH, and 30 µl of different protein amounts each, ranging from 5µl to 30 µl (in six steps; protein concentration unknown because purification was not performed, just a lysis of the cells with TES). All samples were prepared on ice. (In hindsight the possible blank with just NADPH appears to be a non-optimal solution because the auto catalyzation of this chemical likely happens just a few minutes into the assay.)

The 96 well microplate was loaded as depicted in the picture below:

The assay was run for 200 kinetic cycles, each 30 secs long and with 25 photo pulses per cycle. The reader was heated to the appropriate temperature of 37° celsius.

• The 'gre' curve shows the enzymatic activity of GRE3. The curve drops later than the 'k' curve because the active conversion of xylose to xylitol in dependance of NADPH happens at a much quicker rate than the auto catalyzation of NADPH itself.
• The 'k' curve shows the negative control containing just NADPH without GRE3.

The code utilized to render the plots is embedded at the bottom of the page.

R script

This is the script used to plot the results of itaconic acid and xylitol.