Revision as of 03:36, 27 September 2013

Detection of pH Levels

Why use a pH-inducible promoter?

In order to execute the alkalinity response only when it is needed,, it was first necessary to identify pH-inducible promoters that are active at or near pH 5.5 (citation needed). At pH 5.5 or below, the rate of demineralization of the tooth exceeds that of the re-mineralization process provided by saliva (citation needed). This results in erosion of the hard tissues of the tooth (citation needed). Thus, a promoter induced at pH 5.5 provides useful transcriptional control over genes that might prevent the progression of tooth decay.

Identifying a pH-inducible promoter

The E. coli genome contains genes which demonstrate elevated levels of transcription at or near pH 5.5. Tucker, et al. (http://jb.asm.org/content/184/23/6551.full) performed a comprehensive study that identified acid-inducible genes contained within the E. coli genome. The team compared the expression levels of genes in cells grown at pH 5.5 to cells grown in pH 7.4. They found that the transcription of the asr and gadA genes were considerably induced at pH 5.5. In fact, the asr gene was the most significantly pH-induced gene identified. Our team proceeded with isolating the promoters of the asr and gadA genes to be used as the pH-inducible promoters driving elevated levels of gene expression within our dual-state promoter.

GadA is a crucial component in the acid stress response of E. coli

On the other hand, the gadA gene is better-characterized. The gadA gene is a part of the gad system, which is an acid-inducible glutamate decarboxylase-based acid resistance system that enables the survival of E. coli under acid stress conditions. (http://jb.asm.org/content/188/23/8118.full). GadA is a gene encoding a glutamate decarboxylase. (http://jb.asm.org/content/185/15/4644.full, http://jb.asm.org/content/188/23/8118.full) The process of decarboxylating glutamate consumes protons that leach into the cell under acid stress. (http://jb.asm.org/content/188/23/8118.full) In this manner, the gad system manages protons that would otherwise drop the cellular pH below levels at which E. coli could survive.

The function of the gad system explains why these genes experience high transcription levels at low pH. Despite this functional explanation, modes of transcriptional control over the gad system are rather complex. Transcriptional factors RpoS, cyclic AMP receptor protein, HN-S and EvgA all play a role in transcriptional regulation. INCOMPLETE SECTION -Do more research, since this section is complicated.

Identification of gadA and asr promoter regions

Transcriptional regulation of asr promoter

As of yet, the function of the asr gene, or “acid-shock RNA” gene, and the mechanism responsible for its induction are still unclear. However, Iien et al. have taken significant steps toward characterizing the gene. They propose that asr encodes a periplasmic or outer-membrane protein. Knockout experiments illustrated that the PhoBR operon plays a significant role in activating the asr gene. They demonstrated through mobility shift electrophoresis that the PhoB protein binds to the promoter region of asr. By analyzing the sequence of the asr promoter region, they revealed that it contains a sequence similar to that of the Pho box, which is a consensus sequence known to bind the PhoB protein. The Pho box can be found in the promoter regions of other PhoB-regulated genes. (http://jb.asm.org/content/181/7/2084.long)This evidence suggests thatthe regulatory protein PhoB indeed exerts some transcriptional control over the asr gene.

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 <div>
 <h1> Detection of pH Levels </h1>
-<div>
-<p>In order to negate pH drops after meals, we needed a way to detect the surrounding pH. We searched various methods of how different bacteria detect pH. However, we concluded that it would be better to search if E. Coli, our model bacteria, has any inherent mechanisms to detect pH levels. This way we don't need to insert genes that code for the all proteins involved in the pathway since it is already there. We just need to extract the promoter sequence and use it for our plasmid. In <i>Gene Expression Profiling of the pH Response in Escherichia Coli (2002) </i>, certain genes showed increased activity under low pH of 5.5, which is also the pH threshold for tooth enamel demineralization. Below is a table of changed gene expression and the red circles are the genes that had especially strong expression levels.</p>
-<center><img src="https://static.igem.org/mediawiki/2013/d/d0/PH_detection.png" width="600" height="200" />
+<h4>Why use a pH-inducible promoter? </h4>
-<p><font size=1>Figure 1. Statistically significant genes at pH 5.5 The significance was determined as induction ≥3 standard deviations from the mean (no change in expression) & P value of ≤ 0.05 as determined by t-test.</font></p></center>
+<p> In order to execute the alkalinity response only when it is needed,, it was first necessary to identify pH-inducible promoters that are active at or near pH 5.5 (citation needed). <b>At pH 5.5 or below, the rate of demineralization of the tooth exceeds that of the re-mineralization process provided by saliva (citation needed). </b>This results in erosion of the hard tissues of the tooth (citation needed). <b>Thus, a promoter induced at pH 5.5 provides useful transcriptional control over genes that might prevent the progression of tooth decay.</b><p>
+<h4>Identifying a pH-inducible promoter</h4>
+<p>The E. coli genome contains genes which demonstrate elevated levels of transcription at or near pH 5.5. <b>Tucker, et al. (http://jb.asm.org/content/184/23/6551.full) performed a comprehensive study that identified acid-inducible genes contained within the E. coli genome.</b> The team compared the expression levels of genes in cells grown at pH 5.5 to cells grown in pH 7.4. They <b>found that the transcription of the asr and gadA genes were considerably induced at pH 5.5.</b> In fact, the asr gene was the most significantly pH-induced gene identified. <b>Our team proceeded with isolating the promoters of the asr and gadA genes to be used as the pH-inducible promoters driving elevated levels of gene expression within our dual-state promoter.</b></p>
+<h4>GadA is a crucial component in the acid stress response of E. coli</h4>
+     <p>On the other hand, the gadA gene is better-characterized. The gadA gene is a part of the gad system, which is an acid-inducible glutamate decarboxylase-based acid resistance system that enables the survival of E. coli under acid stress conditions. (http://jb.asm.org/content/188/23/8118.full).  <b>GadA is a gene encoding a glutamate decarboxylase.</b> (http://jb.asm.org/content/185/15/4644.full,  http://jb.asm.org/content/188/23/8118.full)<b> The process of decarboxylating glutamate consumes protons that leach into the cell under acid stress. </b>(http://jb.asm.org/content/188/23/8118.full)<b>  In this manner, the gad system manages protons that would otherwise drop the cellular pH below levels at which E. coli could survive.</b></p>
+     <p>The function of the gad system explains why these genes experience high transcription levels at low pH. Despite this functional explanation, modes of transcriptional control over the gad system are rather complex. Transcriptional factors RpoS, cyclic AMP receptor protein, HN-S and EvgA all play a role in transcriptional regulation. INCOMPLETE SECTION -Do more research, since this section is complicated. </p>
+<h4>Identification of gadA and asr promoter regions</h4>
+<h4>Transcriptional regulation of asr promoter</h4>
+      <p><b>As of yet, the function of the asr gene, or “acid-shock RNA” gene, and the mechanism responsible for its induction are still unclear.</b> However, Iien et al. have taken significant steps toward characterizing the gene. They propose that<b> asr encodes a periplasmic or outer-membrane protein.</b> Knockout experiments illustrated that the PhoBR operon plays a significant role in activating the asr gene. They demonstrated through mobility shift electrophoresis that the PhoB protein binds to the promoter region of asr.  By analyzing the sequence of the asr promoter region, they revealed that it contains a sequence similar to that of the Pho box, which is a consensus sequence known to bind the PhoB protein. The Pho box can be found in the promoter regions of other PhoB-regulated genes. (http://jb.asm.org/content/181/7/2084.long)This evidence suggests that<b>the regulatory protein PhoB indeed exerts some transcriptional control over the asr gene. </b></p>
-<p> Out of the three genes (Asr, gadA, and hdeA), Asr and GadA were more isolated compared to hdeA. Our project looked into these two genes for pH detection. Both have different mechanisms of sensing pH. Asr works through the PhoBR operon system.</p>
-<center><img src="https://static.igem.org/mediawiki/2013/b/bc/Asr_mechanism.png" width="600" height="400" />
-<p><font size=1>Figure 2. PhoB, when phosphorylated by PhoR, would form homodimers and bind to the consensus pho-box sequence involved in the corresponding promoter and activate downstream genes expression.</font></p></center>
-<p>For GadA, GadA forms an operon with GadX. GadE activates GadA and GadB. Binding of RcsB and gadE as a heterodimer to the GAD box activates gadA transcription.</p>
-<center><img src="https://static.igem.org/mediawiki/2013/e/e2/GadA.jpg" width="400" height="200" />
-<p><font size=1>Figure 3. GadA Mechanism</font></p></center>
 </div>

Team:Northwestern/detectpH

From 2013.igem.org