Difference between revisions of "Part:BBa K4845017"
 
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X-3-temA-2
 
X-3-temA-2
  
<h3>Construction Design</h3>
 
<p>
 
    Based on BBa_K4000000 (TEF1 promoter), we added the part BBa_K4845004 (GAP promoter), BBa_K4000002 (CYC1 terminator), BBa_K4845007 (ADH1 terminator), and BBa_K4845009 (temA) to BBa_K4845003 (X-3-backbone). The new recombinant plasmid BBa_K4845017
 
    (X-3-temA-2) was constructed to increase two promoters and terminators, two temA genes on the X-3-backbone plasmid, improve the enzyme activity of glucoamylase, and further enhance the ability of yeast to decompose starch.
 
</p>
 
<p>
 
    In order to construct BBa_K4845017 (X-3-temA-2), we first amplified the GAP and TEF1 promoters, temA key genes, and CYC1 and ADH1 terminators through PCR (Table 1). Since we were inserting two temA genes into the same plasmid, we used two different
 
    promoters and two different terminators. With the preparation of basic materials, we linked the promoters, key genes, and terminators together through Over PCR to construct GAP-temA-CYC1 and TEF1-temA-ADH1 genes, which would be inserted into the plasmid
 
    skeletons (X-3) later (Figure 1). The design of our target genes is displayed both in the form of a table and a visualized diagram.
 
</p>
 
  
<figure style="text-align: center;">
+
<html>
     <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/1.png" alt="Figure 1" width="600">
+
<head>
    <figcaption>Figure 1: Visualized blocks-assembly diagram showing our design of the temA DNA template. Upper one: GAP-temA-CYC1 gene of 2804 bp. Lower one: TEF1-temA-CYC1 gene of 2482 bp.</figcaption>
+
  <title>Composite Part BBa_K4845017 (X-3-temA-2)</title>
</figure>
+
</head>
 +
<body>
 +
  <h1>Composite Part BBa_K4845017 (X-3-temA-2)</h1>
 +
  <h2>Construction Design</h2>
 +
  <p>Based on <a href="https://www.igem.org/registry/Part:BBa_K4000000">BBa_K4000000 (TEF1 promoter)</a>, we added the following parts:</p>
 +
  <ul>
 +
     <li><a href="https://www.igem.org/registry/Part:BBa_K4845004">BBa_K4845004 (GAP promoter)</a></li>
 +
    <li><a href="https://www.igem.org/registry/Part:BBa_K4000002">BBa_K4000002 (CYC1 terminator)</a></li>
 +
    <li><a href="https://www.igem.org/registry/Part:BBa_K4845007">BBa_K4845007 (ADH1 terminator)</a></li>
 +
    <li><a href="https://www.igem.org/registry/Part:BBa_K4845009">BBa_K4845009 (temA)</a></li>
 +
  </ul>
 +
  <p>These parts were added to <a href="https://www.igem.org/registry/Part:BBa_K4845003">BBa_K4845003 (X-3-backbone)</a>. The new recombinant plasmid <a href="https://www.igem.org/registry/Part:BBa_K4845017">BBa_K4845017 (X-3-temA-2)</a> was constructed to increase two promoters and terminators, two temA genes on the X-3-backbone plasmid, improve the enzyme activity of glucoamylase, and further improve the ability of yeast to decompose starch.</p>
 +
  <p>In order to construct BBa_K4845017 (X-3-temA-2), we firstly amplified the GAP, TEF1 promoters, temA key genes, and CYC1, ADH1 terminators through PCR (Table 1). Since we would insert two temA genes into the same plasmid, we used two different promoters and two different terminators. With the preparation of basic materials, we linked the promoters, key genes, and terminators together through Over PCR to construct GAP-temA-CYC1 and TEF1-temA-ADH1 genes, which will be inserted into the plasmid skeletons (X-3) later (Figure 1). What is more, the design of our target genes is displayed both in the form of a table and the form of a visualized diagram.</p>
  
<p>
+
  <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/table-1.png" alt="Table 1" width="500">
    After obtaining our target temA gene fragments, we inserted them into X-3 plasmid skeletons using the restriction endonuclease digestion and ligation method (Figure 2).
+
  <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/1.png" alt="Figure 1: visualized blocks-assembly diagram for showing our design of temA DNA template" width="500">
</p>
+
  <p>Figure 1: Visualized blocks-assembly diagram for showing our design of temA DNA template</p>
 +
  <p>Upper one: GAP-temA-CYC1 gene of 2804 bp</p>
 +
  <p>Lower one: TEF1-temA-CYC1 gene of 2482 bp</p>
  
<figure style="text-align: center;">
+
  <p>After we obtained our target temA gene fragments, we inserted them into X-3 plasmid skeletons through restriction endonuclease digestion and ligation method (Figure 2).</p>
    <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/2.png" alt="Figure 2" width="600">
+
    <figcaption>Figure 2: Visualized models of our designed plasmids (X-3-2temA).</figcaption>
+
</figure>
+
  
<h3>Engineering Principle</h3>
+
  <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/2.png" alt="Figure 2: Visualized models of our plasmids designed (X-3-2temA)" width="500">
<p>
+
  <p>Figure 2:  Figure 2 : Visualized models of our plasmids designed (X-3-2temA)</p>
    In alcoholic fermentation, α-amylase cannot hydrolyze α-1,6 glycosidic bonds. The complete hydrolysis of starch requires the synergistic effect of α-amylase and glucoamylase, but α-amylase is considered to be more important than glucoamylase because the hydrolysis
+
  <h2>Engineering Principle</h2>
    of starch into oligosaccharides by α-amylase may be the rate-limiting step. Therefore, the glucoamylase was integrated into the plasmid, and the starch α-1,4 glycosidic bond was rapidly hydrolyzed, while the α-1,6 glycosidic bond and α-1,3 glycosidic
+
  <p>In alcoholic fermentation, α-amylase cannot hydrolyze α-1,6 glycosidic bonds. The complete hydrolysis of starch requires the synergistic effect of α-amylase and glucoamylase, but α-amylase is considered to be more important than glucoamylase, because the hydrolysis of starch into oligosaccharides by α-amylase may be the rate-limiting step. Therefore, the glucoamylase was integrated into the plasmid, and the starch α-1,4 glycosidic bond was rapidly hydrolyzed, and the α-1,6 glycosidic bond and α-1,3 glycosidic bond were slowly hydrolyzed, and the final product was all glucose.</p>
    bond were slowly hydrolyzed, resulting in the final product being all glucose.
+
</p>
+
  
<h3>Characterization/Measurement</h3>
+
  <h2>Characterization/Measurement</h2>
 +
  <h3>A. DNA sequencing of X-3-temA plasmid</h3>
 +
  <p>According to the sequencing diagram shown, our X-3-temA and X-3-temA-2 plasmids were constructed successfully (Figure 3 and 4).</p>
 +
  <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/3.png" alt="Figure 3: DNA sequencing result of X-3-temA plasmid" width="500">
 +
  <p>Figure 3: DNA sequencing result of X-3-temA plasmid</p>
 +
  <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/4.png" alt="Figure 4: DNA sequencing result of X-3-temA-2 plasmid" width="500">
 +
  <p>Figure 4: DNA sequencing result of X-3-temA-2 plasmid</p>
  
<p>A. DNA sequencing of X-3-temA plasmid</p>
+
  <h3>B. Transformation testing of temA-containing plasmids through PCR and Gel electrophoresis</h3>
<p>
+
  <p>The figure 5 shown in figure A leads to the length of temA genes fragment of X-3 plasmid. We have successfully constructed those plasmids and we are able to confirm that we have successfully transformed our constructed temA-containing plasmid into 1974 yeast cells.</p>
    According to the sequencing diagram shown, our X-3-temA and X-3-temA-2 plasmids were constructed successfully (Figure 3 and 4).
+
  <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/5.png" alt="Figure 5: Results of PCR of plasmids extracted from temA-genes-containing 1974 yeast cell" width="500">
</p>
+
  <p>Figure 5: Results of PCR of plasmids extracted from temA-genes-containing 1974 yeast cell</p>
 +
</body>
 +
</html>
  
<figure style="text-align: center;">
 
    <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/3.png" alt="Figure 3" width="600">
 
    <figcaption>Figure 3: DNA sequencing result of X-3-temA plasmid.</figcaption>
 
</figure>
 
 
<figure style="text-align: center;">
 
    <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/4.png" alt="Figure 4" width="600">
 
    <figcaption>Figure 4: DNA sequencing result of X-3-temA-2 plasmid.</figcaption>
 
</figure>
 
 
<p>B. Transformation testing of temA-containing plasmids through PCR and Gel electrophoresis</p>
 
<p>
 
    Figure 5 shows the length of temA gene fragments of X-3 plasmid. We have successfully constructed those plasmids, and we are able to confirm that we have successfully transformed our constructed temA-containing plasmid into 1974 yeast cells.
 
</p>
 
 
<figure style="text-align: center;">
 
    <img src="https://static.igem.wiki/teams/4845/wiki/bba-k4845017/5.png" alt="Figure 5" width="600">
 
    <figcaption>Figure 5: Results of PCR of plasmids extracted from temA-genes-containing 1974 yeast cells.</figcaption>
 
</figure>
 
  
  

Latest revision as of 14:03, 9 October 2023


X-3-temA-2

X-3-temA-2


Composite Part BBa_K4845017 (X-3-temA-2)

Composite Part BBa_K4845017 (X-3-temA-2)

Construction Design

Based on BBa_K4000000 (TEF1 promoter), we added the following parts:

These parts were added to BBa_K4845003 (X-3-backbone). The new recombinant plasmid BBa_K4845017 (X-3-temA-2) was constructed to increase two promoters and terminators, two temA genes on the X-3-backbone plasmid, improve the enzyme activity of glucoamylase, and further improve the ability of yeast to decompose starch.

In order to construct BBa_K4845017 (X-3-temA-2), we firstly amplified the GAP, TEF1 promoters, temA key genes, and CYC1, ADH1 terminators through PCR (Table 1). Since we would insert two temA genes into the same plasmid, we used two different promoters and two different terminators. With the preparation of basic materials, we linked the promoters, key genes, and terminators together through Over PCR to construct GAP-temA-CYC1 and TEF1-temA-ADH1 genes, which will be inserted into the plasmid skeletons (X-3) later (Figure 1). What is more, the design of our target genes is displayed both in the form of a table and the form of a visualized diagram.

Table 1 Figure 1: visualized blocks-assembly diagram for showing our design of temA DNA template

Figure 1: Visualized blocks-assembly diagram for showing our design of temA DNA template

Upper one: GAP-temA-CYC1 gene of 2804 bp

Lower one: TEF1-temA-CYC1 gene of 2482 bp

After we obtained our target temA gene fragments, we inserted them into X-3 plasmid skeletons through restriction endonuclease digestion and ligation method (Figure 2).

Figure 2: Visualized models of our plasmids designed (X-3-2temA)

Figure 2: Figure 2 : Visualized models of our plasmids designed (X-3-2temA)

Engineering Principle

In alcoholic fermentation, α-amylase cannot hydrolyze α-1,6 glycosidic bonds. The complete hydrolysis of starch requires the synergistic effect of α-amylase and glucoamylase, but α-amylase is considered to be more important than glucoamylase, because the hydrolysis of starch into oligosaccharides by α-amylase may be the rate-limiting step. Therefore, the glucoamylase was integrated into the plasmid, and the starch α-1,4 glycosidic bond was rapidly hydrolyzed, and the α-1,6 glycosidic bond and α-1,3 glycosidic bond were slowly hydrolyzed, and the final product was all glucose.

Characterization/Measurement

A. DNA sequencing of X-3-temA plasmid

According to the sequencing diagram shown, our X-3-temA and X-3-temA-2 plasmids were constructed successfully (Figure 3 and 4).

Figure 3: DNA sequencing result of X-3-temA plasmid

Figure 3: DNA sequencing result of X-3-temA plasmid

Figure 4: DNA sequencing result of X-3-temA-2 plasmid

Figure 4: DNA sequencing result of X-3-temA-2 plasmid

B. Transformation testing of temA-containing plasmids through PCR and Gel electrophoresis

The figure 5 shown in figure A leads to the length of temA genes fragment of X-3 plasmid. We have successfully constructed those plasmids and we are able to confirm that we have successfully transformed our constructed temA-containing plasmid into 1974 yeast cells.

Figure 5: Results of PCR of plasmids extracted from temA-genes-containing 1974 yeast cell

Figure 5: Results of PCR of plasmids extracted from temA-genes-containing 1974 yeast cell


Sequence and Features


Assembly Compatibility:
  • 10
    COMPATIBLE WITH RFC[10]
  • 12
    INCOMPATIBLE WITH RFC[12]
    Illegal NotI site found at 3656
    Illegal NotI site found at 4104
  • 21
    INCOMPATIBLE WITH RFC[21]
    Illegal XhoI site found at 3877
    Illegal XhoI site found at 6026
    Illegal XhoI site found at 8750
  • 23
    COMPATIBLE WITH RFC[23]
  • 25
    INCOMPATIBLE WITH RFC[25]
    Illegal AgeI site found at 6263
    Illegal AgeI site found at 6697
    Illegal AgeI site found at 8987
  • 1000
    INCOMPATIBLE WITH RFC[1000]
    Illegal BsaI site found at 2651
    Illegal BsaI.rc site found at 132
    Illegal BsaI.rc site found at 4399
    Illegal SapI site found at 284
    Illegal SapI site found at 4213
    Illegal SapI.rc site found at 1629
    Illegal SapI.rc site found at 4636