Latest revision as of 19:50, 4 October 2013

Aerobic consumption of ammonium and hydroxylamine

Introduction

In this aerobic experiment, we add ammonium NH₄⁺ to AMO transformed E. coli cells and measure the consumption of ammonium to determine whether our AMO transformant is converting ammonium to hydroxylamine (NH₂OH) faster than an untransformed E. coli control. A similar protocol is used to determine whether our HAO transformant is converting hydroxylamine to nitrite NO₂^-, by measuring production of nitrite.

Methods

The experiment is based on the protocol Experiment 4 and it was performed on August 27^th and August 28^th.

Results

AMO Transformant

Ammonia measured plotted vs optical density from minutes 129 to 885 for two replicates of the AMO transformant, and an untransformed E. coli control. The slope (change in concentration of Ammonia / change in optical density) of this graph indicates consumption of Ammonia.

Strain	d[NH₄⁺]/dOD
AMO replicate 1	-479.3
AMO replicate 2	-356.2
E. coli	-103.2

Supplemental figures follow.

HAO Transformant

Over the course of the experiment, the OD for all treatments that hydroxylamine was added to decreased or remained essentially constant. Additionally, no nitrite was detected in any of the treatments.

Conclusion and Discussion

The AMO transformant uses ammonia at a rate greater than the untransformed E. coli control. This suggests that the AMO is consuming ammonia and converting it to hydroxylamine. Additionally, however, the AMO transformant grows significantly more slowly than the control.

It is clear that hydroxylamine is toxic to the cells at this concentration. With more time, it would be interesting to repeat the toxicity experiment using hydroxylamine to determine the threshold concentration that causes cell death. We expect that in vivo, the hydroxylamine to nitrite reaction catalyzed by HAO happens very quickly and that even at high throughput, hydroxylamine should not accumulate in the cell.

@@ Line 8: / Line 8: @@
 == Methods ==
-The experiment is based on the protocol [[Team:DTU-Denmark/Methods/Determining_concentration_of_nitrogen_compounds/Experiment_4|Experiment 4]] and it was performed at [[Team:DTU-Denmark/Notebook/27_August_2013#lab_115| August 27<sup>th</sup>]] and [[Team:DTU-Denmark/Notebook/28_August_2013#lab_115|August 28<sup>th</sup>]].
+The experiment is based on the protocol [[Team:DTU-Denmark/Methods/Determining_concentration_of_nitrogen_compounds/Experiment_4|Experiment 4]] and it was performed on [[Team:DTU-Denmark/Notebook/27_August_2013#lab_115| August 27<sup>th</sup>]] and [[Team:DTU-Denmark/Notebook/28_August_2013#lab_115|August 28<sup>th</sup>]].
 == Results ==
@@ Line 18: / Line 18: @@
 Ammonia measured plotted vs optical density from minutes 129 to 885 for two replicates of the AMO transformant, and an untransformed ''E. coli'' control.  The slope (change in concentration of Ammonia / change in optical density) of this graph indicates consumption of Ammonia.
-{|
+{| class="wikitable"
 ! Strain
 ! d[NH<sub>4</sub><sup>+</sup>]/dOD
 |-
-|AMO1
+|AMO replicate 1
-|
+| -479.3
 |-
-|AMO2
+|AMO replicate 2
-|
+| -356.2
 |-
 |''E. coli''
-|
+| -103.2
 |-
 |}
@@ Line 52: / Line 52: @@
 It is clear that hydroxylamine is toxic to the cells at this concentration.  With more time, it would be interesting to repeat the [[Team:DTU-Denmark/ToxicityExperiment|toxicity experiment]] using hydroxylamine to determine the threshold concentration that causes cell death.  We expect that ''in vivo'', the hydroxylamine to nitrite reaction catalyzed by HAO
-happens very quickly (TODO add ref) and that even at high throughput, hydroxylamine should not accumulate in the cell.
+happens very quickly and that even at high throughput, hydroxylamine should not accumulate in the cell.
 <div style="clear: both;"></div>
 {{:Team:DTU-Denmark/Templates/EndPage}}

Team:DTU-Denmark/Experiment4

From 2013.igem.org