Difference between revisions of "Part:BBa K4759020"

Latest revision as of 06:11, 12 October 2023

hemA

A gene coding for glutamyl-tRNA reductase (GluTR),Glutamyl-tRNA reductase catalyzes the first step of porphyrin biosynthesis. Forms part of the pathway for the biosynthesis of 5-aminolevulinate from glutamate, known as the C5 pathway, which is used in most eubacteria, and in all archaebacteria, algae and plants.

(S)-4-amino-5-oxopentanoate + NADP⁽⁺⁾ + tRNA(Glu) <=> H⁽⁺⁾ + L-glutamyl-tRNA(Glu) + NADPH

Design

We cloned this gene and constructed the recombinant plasmid pCDFDuet-hemA-hemL to express hemA in engineered bacteria

Usage and Biology

We divided the synthesis pathway of heme into two parts, one is the synthesis pathway of heme premise ALA (upstream), and the other part is the synthesis pathway of ALA to heme (downstream). For the upstream pathway, there were two pathways from glutamate to ALA, one was the C4 pathway and the other was the C5 pathway. The C4 pathway had been enhanced by the existing team, and the experimental results showed that the effect was not as good as the C5 pathway, so we chose the C5 pathway for modification. The C5 pathway had two key genes, one was hemA and the other was hemL. So we constructed plasmids containing hemA and hemL, and overexpressed them by transforming recombinant plasmids to E. coli. The downstream pathway, that was, the synthesis pathway of heme, involved 7 genes, of which 4 genes (hemB, hemD, hemC, hemH) were more critical, according to the literature. Therefore, we also constructed and overexpressed plasmids containing hemB , hemD, hemC , and hemH .

Fig2: Heme biosynthetic pathways in E. coli . The purple arrow represents the C5 pathway and the pink arrow represents the downstream biosynthetic pathway of heme. The pCDFDuet-hemA-hemL plasmid was constructed to enhance C5 pathway; the pETDuet-hemBDC-hemH plasmid was constructed to enhance downstream biosynthetic pathway

Therefore, 3 recombinant strains were constructed, E. coli AL strain(The recombinant plasmid pCDFDuet-hemA-hemL was expressed in E. coli O2), E. coli BCDH strain (The recombinant plasmid pETDuet-hemB-hemC-hemD-hemH was expressed in E. coliO2), E. coli AL-BCDH strain(The recombinant plasmids pCDFDuet-hemA-hemL and pETDuet-hemB-hemC-hemD-hemH were expressed in E. coli O2).

Fig3: The color of engineered strains and pure enzyme. 1: E. coli O1 strain; 2: E. coli O2 strain; 3: E. coli O2 strain cultivated with ALA and FeCl_{3_{; 4: E. coli AL strain; 5: Olep enzyme purified from E. coliAL strain. The lower values represent the content of intracellular heme in different engineered strains}}

The experimental results showed that, without the addition of ALA and FeCl_{3_{, the heme binding rate of Olep increased to 53.9%, and the conversion rate of deoxycholic acid increased to 41.4%.}}

Fig4: The effect of enhancing heme biosynthesis on the Olep catalysis

Sequence and Features

Assembly Compatibility:

10
COMPATIBLE WITH RFC[10]
12
COMPATIBLE WITH RFC[12]
21
INCOMPATIBLE WITH RFC[21]
Illegal BglII site found at 246
Illegal BglII site found at 524
23
COMPATIBLE WITH RFC[23]
25
COMPATIBLE WITH RFC[25]
1000
INCOMPATIBLE WITH RFC[1000]
Illegal SapI.rc site found at 178

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 <partinfo>BBa_K4759020 short</partinfo>
-the insufficient supply of heme limits the whole-cell P450 biocatalytic activity.A gene coding for  glutamyl-tRNA reductase (GluTR),Glutamyl-tRNA reductase catalyzes the first step of porphyrin biosynthesis. Forms part of the pathway for the biosynthesis of 5-aminolevulinate from glutamate, known as the C5 pathway, which is used in most eubacteria, and in all archaebacteria, algae and plants.
+A gene coding for glutamyl-tRNA reductase (GluTR),Glutamyl-tRNA reductase catalyzes the first step of porphyrin biosynthesis. Forms part of the pathway for the biosynthesis of 5-aminolevulinate from glutamate, known as the C5 pathway, which is used in most eubacteria, and in all archaebacteria, algae and plants.
-(S)-4-amino-5-oxopentanoate + NADP(+) + tRNA(Glu) <=> H(+) + L-glutamyl-tRNA(Glu) + NADPH
-===Design Notes===
+(S)-4-amino-5-oxopentanoate + NADP<sup>(+)</sup> + tRNA(Glu) <=> H<sup>(+)</sup> + L-glutamyl-tRNA(Glu) + NADPH
-Recombinant plasmid pCDFDuet-hemA-hemL is expressed in engineered bacteria
-===Applications of BBa_K4759020===
+===Design===
-First, three different combinations of exogenous additions (direct addition of Heme, addition of precursor ALA+FeSO4, addition of precursor ALA+FeCl3) are tested. The results showed that the addition of 0.64 mM ALA and 0.3 mM FeCl3 during the induction of Olep increased the heme binding rate to 67.7% and the conversion rate of deoxycholic acid to 40.7%. Through the above experiments, we verified that the increase in heme content has a positive effect on P450 enzyme activity, but the exogenous addition of ALA increases the cost of whole-cell catalysis by 60%, so we tried to increase intracellular heme content by strengthening the heme synthesis pathway of
-E. coli itself.
-https://static.igem.wiki/teams/4759/wiki/hem4.png
+We cloned this gene and constructed the recombinant plasmid pCDFDuet-hemA-hemL to express <i>hemA</i> in engineered bacteria
-Fig3-2: The effect of supplements on the Olep catalysis
+===Usage and Biology===
-.3 Endogenous synthesis of heme
+We divided the synthesis pathway of heme into two parts, one is the synthesis pathway of heme premise ALA (upstream), and the other part is the synthesis pathway of ALA to heme (downstream).
+For the upstream pathway, there were two pathways from glutamate to ALA, one was the C4 pathway and the other was the C5 pathway. The C4 pathway had been enhanced by the existing team, and the experimental results showed that the effect was not as good as the C5 pathway, so we chose the C5 pathway for modification. The C5 pathway had two key genes, one was <i>hemA</i> and the other was <i>hemL</i>. So we constructed plasmids containing hemA and hemL, and overexpressed them by transforming recombinant plasmids to E. coli.
-We divide the synthesis pathway of heme into two parts, one is the synthesis pathway of heme premise ALA, and the other part is the synthesis pathway of ALA to heme, one upstream and one downstream.
+The downstream pathway, that was, the synthesis pathway of heme, involved 7 genes, of which 4 genes (<i>hemB</i>, <i>hemD</i>, <i>hemC</i>, <i>hemH</i>) were more critical, according to the literature. Therefore, we also constructed and overexpressed plasmids containing <i>hemB</i> , <i> hemD</i>, <i>hemC</i> , and <i>hemH</i> .
-For the upstream pathway, there are two pathways from glutamate to ALA, one is the C4 pathway and the other is the C5 pathway. The C4 pathway has been enhanced by the existing team, and the experimental results show that the effect is not as good as the C5 pathway, so we chose the C5 pathway for modification. The C5 pathway has two key genes, one is hemA and the other is hemL. By constructing plasmid containing hemA and hemL and transforming them, we overexpress hemA and hemL genes.
-The downstream pathway, that is, the synthesis pathway of heme, involves 7 genes, of which 4 genes (hemB, hemD, hemC, hemH) are more critical, according to the literature. Therefore, we also constructed plasmid to overexpress hemB, D, C, and H.
 https://static.igem.wiki/teams/4759/wiki/hem.png
-Fig3-3: Heme biosynthetic pathways in E. coli. The purple arrow represents the C5 pathway and the pink arrow represents the downstream biosynthetic pathway of heme. The pCDFDuet-hemA-hemL plasmid was constructed to enhance C5 pathway; the pETDuet-hemBDC-hemH plasmid was constructed to enhance downstream biosynthetic pathway
+Fig2: Heme biosynthetic pathways in <i>E. coli</i> . The purple arrow represents the C5 pathway and the pink arrow represents the downstream biosynthetic pathway of heme. The pCDFDuet-hemA-hemL plasmid was constructed to enhance C5 pathway; the pETDuet-hemBDC-hemH plasmid was constructed to enhance downstream biosynthetic pathway
-Therefore, 3 recombinant strains are constructed, E. coli AL strain(The recombinant plasmid pCDFDuet-hemA-hemL is expressed in E. coli O2), E. coli BCDH strain (The recombinant plasmid pETDuet-hemB-hemC-hemD-hemH is expressed in E. coli O2), E. coli AL-BCDH strain(The recombinant plasmids pCDFDuet-hemA-hemL and pETDuet-hemB-hemC-hemD-hemH are expressed in E. coli O2).
+Therefore, 3 recombinant strains were constructed, <i>E. coli</i> AL strain(The recombinant plasmid pCDFDuet-hemA-hemL was expressed in <i>E. coli</i> O2), <i>E. coli</i> BCDH strain (The recombinant plasmid pETDuet-hemB-hemC-hemD-hemH was expressed in <i>E. coli</i>O2), <i>E. coli</i> AL-BCDH strain(The recombinant plasmids pCDFDuet-hemA-hemL and pETDuet-hemB-hemC-hemD-hemH were expressed in <i>E. coli</i> O2).
 https://static.igem.wiki/teams/4759/wiki/hem2.png
-Fig3-4: The color of engineered strains and pure enzyme. 1: E. coli O1 strain; 2: E. coli O2 strain; 3: E. coli O2 strain cultivated with ALA and FeCl3; 4: E. coli AL strain; 5: Olep enzyme purified from E. coli AL strain. The lower values represent the content of intracellular heme in different engineered strains
+Fig3: The color of engineered strains and pure enzyme. 1: <i>E. coli</i> O1 strain; 2: <i>E. coli</i> O2 strain; 3: <i>E. coli</i> O2 strain cultivated with ALA and FeCl<sub>3<sub>; 4: <i>E. coli</i> AL strain; 5: Olep enzyme purified from <i>E. coli</i>AL strain. The lower values represent the content of intracellular heme in different engineered strains
-The experimental results showed that, without the addition of ALA and FeCl3, the heme binding rate of Olep increased to 53.9%, and the conversion rate of deoxycholic acid increased to 41.4%.
+The experimental results showed that, without the addition of ALA and FeCl<sub>3<sub>, the heme binding rate of Olep increased to 53.9%, and the conversion rate of deoxycholic acid increased to 41.4%.
 https://static.igem.wiki/teams/4759/wiki/hem3.png
-Fig3-5: The effect of enhancing heme biosynthesis on the Olep catalysis
+Fig4: The effect of enhancing heme biosynthesis on the Olep catalysis
 <!-- Add more about the biology of this part here
-===Usage and Biology===