Difference between revisions of "Part:BBa K5216000"
(→Conclusion) |
|||
(2 intermediate revisions by the same user not shown) | |||
Line 3: | Line 3: | ||
<partinfo>BBa_K5216000 short</partinfo> | <partinfo>BBa_K5216000 short</partinfo> | ||
− | This part focuses on the synthesis of a β-agarase (AgaA). AgaA specifically cleaves the β-1,4 glycosidic bond between D-galactose and 3,6-anhydro-α-L-galactose residues in agarose, generating neoagarooligosaccharides (NAOS). The gene sequence of AgaA is derived from Marinimicrobium sp. H1 and has been codon-optimized for the E. coli host to enhance expression efficiency in a heterologous expression system[1]. | + | This part focuses on the synthesis of a β-agarase (AgaA). AgaA specifically cleaves the β-1,4 glycosidic bond between D-galactose and 3,6-anhydro-α-L-galactose residues in agarose, generating neoagarooligosaccharides (NAOS). The gene sequence of AgaA is derived from ''"Marinimicrobium'' sp. H1 and has been codon-optimized for the ''E. coli'' host to enhance expression efficiency in a heterologous expression system[1]. |
<!-- Add more about the biology of this part here | <!-- Add more about the biology of this part here | ||
Line 26: | Line 26: | ||
=Design= | =Design= | ||
− | We designed a prokaryotic expression system to express β-agarase AgaA (BBa_K5216000) (Fig.1). In our experiment, we constructed the AgaA_pET-32a(+) prokaryotic expression vector using double-enzyme digestion techniques. After successfully constructing the vector, the recombinant expression vector was transformed into E. coli Rosetta for subsequent protein expression(Fig.2). | + | We designed a prokaryotic expression system to express β-agarase AgaA (BBa_K5216000) (Fig.1). In our experiment, we constructed the AgaA_pET-32a(+) prokaryotic expression vector using double-enzyme digestion techniques. After successfully constructing the vector, the recombinant expression vector was transformed into ''E. coli'' Rosetta for subsequent protein expression(Fig.2). |
<p style="text-align: center;"> | <p style="text-align: center;"> | ||
Line 42: | Line 42: | ||
=Characterization= | =Characterization= | ||
==Protein expression== | ==Protein expression== | ||
− | AgaA_pET-32a (+) plasmid was transformed into ''E. coli'' Rosetta for expression. We induced expression at 16°C for 18 hours with IPTG at a final concentration of 0.5 mM. Protein expression was detected using SDS-PAGE, and Fig. | + | AgaA_pET-32a (+) plasmid was transformed into ''E. coli'' Rosetta for expression. We induced expression at 16°C for 18 hours with IPTG at a final concentration of 0.5 mM. Protein expression was detected using SDS-PAGE, and Fig. 3A demonstrates that the target protein was successfully expressed and that the soluble protein can be used for subsequent experiments. The concentration of AgaA before purification was determined using the Bradford assay, resulting in a final protein concentration of 3.09 mg/mL and a total yield of 61.8 mg, which will be used for subsequent production of the neoagaroligosaccharides NAOS. The expression strain was then scaled up to 100 mL to express the protein, which was purified using Ni-NTA affinity chromatography (Fig. 3B). The figure indicates that the target protein can be purified using this method, with the wash buffer being chosen as 100 mM imidazole buffer and the elution buffer as 300 mM imidazole buffer. |
<p style="text-align: center;"> | <p style="text-align: center;"> | ||
Line 49: | Line 49: | ||
<p style="text-align: center;"><i>Fig. 3 Expression and purification of AgaA.</i></p> | <p style="text-align: center;"><i>Fig. 3 Expression and purification of AgaA.</i></p> | ||
− | <i>(A) AgaA Protein Expression. M: marker; 1, ''E. coli'' Rosetta AgaA_pET-32a(+) culture (without IPTG); 2, ''E. coli'' Rosetta AgaA_pET-32a(+) culture (with IPTG at a final concentration of 0. | + | <i>(A) AgaA Protein Expression. M: marker; 1, ''E. coli'' Rosetta AgaA_pET-32a(+) culture (without IPTG); 2, ''E. coli'' Rosetta AgaA_pET-32a(+) culture (with IPTG at a final concentration of 0.5 mM); 3, ''E. coli'' Rosetta AgaA_pET-32a(+) soluble protein; 4, ''E. coli'' Rosetta AgaA_pET-32a(+) inclusion body. (B) AgaA Protein Purification. M: marker; AgaA (0.5 mM): 1, ''E. coli'' Rosetta AgaA_pET-32a(+) culture (without IPTG); 2, supernatant; 3, 0 mM imidazole; 4, 50 mM imidazole; 5, 100 mM imidazole; 6, 150 mM imidazole; 7, 200 mM imidazole; 8, 300 mM imidazole.</i> |
==Enzyme activity verification== | ==Enzyme activity verification== | ||
− | As observed in Fig. | + | As observed in Fig. 4A, depressions appeared on the LB solid medium where the ''E. coli'' Rosetta AgaA_pET-32a(+) strain was cultured, indicating that this expression strain is capable of degrading agar, thereby demonstrating agarase activity. After inducing expression in this strain, the AgaA enzyme was obtained, and further enzyme activity verification is required. A mixture of 200 µl of AgaA and 200 µl of agarose (2%) was incubated in a 55°C metal bath for 30 minutes. The reaction was then terminated by heating at 95°C for 10 minutes. Next, 200 µl of the reaction mixture was transferred to a new 2 mL EP tube, and 200 µl of DNS reagent was added and mixed. The mixture was heated in a 95°C metal bath for 5 minutes (the control group used pre-inactivated AgaA). The color change between the control group and the experimental group was observed. As shown in Fig. 4B, the color of the experimental group significantly darkened, indicating the production of reducing sugars, specifically NAOS, in the reaction. This experimental result confirms that the heterologously expressed AgaA in ''E. coli'' has biological activity. |
<p style="text-align: center;"> | <p style="text-align: center;"> | ||
Line 57: | Line 57: | ||
</p> | </p> | ||
+ | <p style="text-align: center;"><i>Fig. 4 Analysis of AgaA Enzyme Activity</i></p> | ||
<i>(A)Growth of the AgaA expression strain on LB agar plates. (B) AgaA enzyme activity assay using the DNS method (left: experimental group; right: control group).</i> | <i>(A)Growth of the AgaA expression strain on LB agar plates. (B) AgaA enzyme activity assay using the DNS method (left: experimental group; right: control group).</i> | ||
− | The agarose hydrolysis products are displayed in Fig. | + | The agarose hydrolysis products are displayed in Fig. 5. The standard sample consisted of a mixture of neoagarobiose (NA2), neoagarotetraose (NA4), and neoagarohexaose (NA6), with retention times of 6.75 minutes, 12.4 minutes, and 23.5 minutes, respectively. Upon comparing the chromatograms of the experimental group with the control group, new product peaks appeared at 6.75 minutes and 12.4 minutes following hydrolysis by the AgaA enzyme, indicating that the primary products of this reaction are NA2 and NA4. |
Earlier experiments revealed that AgaA hydrolyzes agarose into NA2, NA4, and NA6, but over time, NA6 is progressively broken down into NA2 and NA4. This demonstrates that the enzyme reaction was quite thorough, as NA6 was fully hydrolyzed into NA2 and NA4. | Earlier experiments revealed that AgaA hydrolyzes agarose into NA2, NA4, and NA6, but over time, NA6 is progressively broken down into NA2 and NA4. This demonstrates that the enzyme reaction was quite thorough, as NA6 was fully hydrolyzed into NA2 and NA4. | ||
Line 69: | Line 70: | ||
==Analysis of oxidation resistance of AgaA hydrolysate== | ==Analysis of oxidation resistance of AgaA hydrolysate== | ||
− | In this experiment, the antioxidant properties of NAOS, the hydrolysis products of AgaA, were evaluated using the ABTS assay. ABTS, when oxidized, forms a stable blue-green cation radical known as ABTS+, which is soluble in aqueous or acidic ethanol solutions | + | In this experiment, the antioxidant properties of NAOS, the hydrolysis products of AgaA, were evaluated using the ABTS assay. ABTS, when oxidized, forms a stable blue-green cation radical known as ABTS+, which is soluble in aqueous or acidic ethanol solutions. When an antioxidant is introduced to the ABTS+ solution, it reacts with the radical, causing a reduction in color intensity. |
− | As illustrated in Fig. | + | As illustrated in Fig. 6, the antioxidant detection reagent containing the AgaA hydrolysis products exhibited a significant decolorization effect compared to the control group. This demonstrates that the NAOS generated from the AgaA-mediated hydrolysis of agarose possess significant antioxidant activity. |
<p style="text-align: center;"> | <p style="text-align: center;"> | ||
Line 76: | Line 77: | ||
</p> | </p> | ||
− | <i>Fig. 6 Antioxidant activity analysis of AgaA hydrolysate.</i> | + | <p style="text-align: center;"><i>Fig. 6 Antioxidant activity analysis of AgaA hydrolysate.</i></p> |
+ | |||
=Conclusion= | =Conclusion= |
Latest revision as of 07:25, 30 September 2024
AgaA (β-agarase)
This part focuses on the synthesis of a β-agarase (AgaA). AgaA specifically cleaves the β-1,4 glycosidic bond between D-galactose and 3,6-anhydro-α-L-galactose residues in agarose, generating neoagarooligosaccharides (NAOS). The gene sequence of AgaA is derived from "Marinimicrobium sp. H1 and has been codon-optimized for the E. coli host to enhance expression efficiency in a heterologous expression system[1].
Sequence and Features
- 10COMPATIBLE WITH RFC[10]
- 12INCOMPATIBLE WITH RFC[12]Illegal NheI site found at 1129
- 21INCOMPATIBLE WITH RFC[21]Illegal XhoI site found at 198
- 23COMPATIBLE WITH RFC[23]
- 25INCOMPATIBLE WITH RFC[25]Illegal NgoMIV site found at 339
Illegal AgeI site found at 577 - 1000INCOMPATIBLE WITH RFC[1000]Illegal BsaI site found at 384
Illegal BsaI site found at 985
Illegal SapI site found at 89
Illegal SapI site found at 221
Illegal SapI site found at 284
Illegal SapI.rc site found at 1066
Introduction
The goal of our project is to develop a novel antioxidant that can remove excess ROS produced in the skin due to environmental factors such as air pollution, UV radiation, and pathogenic microorganisms. This antioxidant will be applied in skincare products to help the skin resist oxidative stress, thereby slowing down aging. To achieve this goal, we have constructed a basic component, AgaA (BBa_K5216000). AgaA efficiently hydrolyzes agarose to generate NAOS, which exhibits high antioxidant activity and is a potential ingredient for skincare products.
Contents
1. Introduction 2. Design 3. Characterization 3.1 Protein expression 3.2 Enzyme activity verification 3.3 Analysis of oxidation resistance of AgaA hydrolysate 4. Conclusion 5. Reference
Design
We designed a prokaryotic expression system to express β-agarase AgaA (BBa_K5216000) (Fig.1). In our experiment, we constructed the AgaA_pET-32a(+) prokaryotic expression vector using double-enzyme digestion techniques. After successfully constructing the vector, the recombinant expression vector was transformed into E. coli Rosetta for subsequent protein expression(Fig.2).
Fig.1 Plasmid map of AgaA_pET-32a(+).
Fig.2 AgaA allogeneic expression diagram.
Characterization
Protein expression
AgaA_pET-32a (+) plasmid was transformed into E. coli Rosetta for expression. We induced expression at 16°C for 18 hours with IPTG at a final concentration of 0.5 mM. Protein expression was detected using SDS-PAGE, and Fig. 3A demonstrates that the target protein was successfully expressed and that the soluble protein can be used for subsequent experiments. The concentration of AgaA before purification was determined using the Bradford assay, resulting in a final protein concentration of 3.09 mg/mL and a total yield of 61.8 mg, which will be used for subsequent production of the neoagaroligosaccharides NAOS. The expression strain was then scaled up to 100 mL to express the protein, which was purified using Ni-NTA affinity chromatography (Fig. 3B). The figure indicates that the target protein can be purified using this method, with the wash buffer being chosen as 100 mM imidazole buffer and the elution buffer as 300 mM imidazole buffer.
Fig. 3 Expression and purification of AgaA.
(A) AgaA Protein Expression. M: marker; 1, E. coli Rosetta AgaA_pET-32a(+) culture (without IPTG); 2, E. coli Rosetta AgaA_pET-32a(+) culture (with IPTG at a final concentration of 0.5 mM); 3, E. coli Rosetta AgaA_pET-32a(+) soluble protein; 4, E. coli Rosetta AgaA_pET-32a(+) inclusion body. (B) AgaA Protein Purification. M: marker; AgaA (0.5 mM): 1, E. coli Rosetta AgaA_pET-32a(+) culture (without IPTG); 2, supernatant; 3, 0 mM imidazole; 4, 50 mM imidazole; 5, 100 mM imidazole; 6, 150 mM imidazole; 7, 200 mM imidazole; 8, 300 mM imidazole.
Enzyme activity verification
As observed in Fig. 4A, depressions appeared on the LB solid medium where the E. coli Rosetta AgaA_pET-32a(+) strain was cultured, indicating that this expression strain is capable of degrading agar, thereby demonstrating agarase activity. After inducing expression in this strain, the AgaA enzyme was obtained, and further enzyme activity verification is required. A mixture of 200 µl of AgaA and 200 µl of agarose (2%) was incubated in a 55°C metal bath for 30 minutes. The reaction was then terminated by heating at 95°C for 10 minutes. Next, 200 µl of the reaction mixture was transferred to a new 2 mL EP tube, and 200 µl of DNS reagent was added and mixed. The mixture was heated in a 95°C metal bath for 5 minutes (the control group used pre-inactivated AgaA). The color change between the control group and the experimental group was observed. As shown in Fig. 4B, the color of the experimental group significantly darkened, indicating the production of reducing sugars, specifically NAOS, in the reaction. This experimental result confirms that the heterologously expressed AgaA in E. coli has biological activity.
Fig. 4 Analysis of AgaA Enzyme Activity
(A)Growth of the AgaA expression strain on LB agar plates. (B) AgaA enzyme activity assay using the DNS method (left: experimental group; right: control group).
The agarose hydrolysis products are displayed in Fig. 5. The standard sample consisted of a mixture of neoagarobiose (NA2), neoagarotetraose (NA4), and neoagarohexaose (NA6), with retention times of 6.75 minutes, 12.4 minutes, and 23.5 minutes, respectively. Upon comparing the chromatograms of the experimental group with the control group, new product peaks appeared at 6.75 minutes and 12.4 minutes following hydrolysis by the AgaA enzyme, indicating that the primary products of this reaction are NA2 and NA4. Earlier experiments revealed that AgaA hydrolyzes agarose into NA2, NA4, and NA6, but over time, NA6 is progressively broken down into NA2 and NA4. This demonstrates that the enzyme reaction was quite thorough, as NA6 was fully hydrolyzed into NA2 and NA4.
Fig. 5 HPLC Analysis of the AgaA Reaction Product
Analysis of oxidation resistance of AgaA hydrolysate
In this experiment, the antioxidant properties of NAOS, the hydrolysis products of AgaA, were evaluated using the ABTS assay. ABTS, when oxidized, forms a stable blue-green cation radical known as ABTS+, which is soluble in aqueous or acidic ethanol solutions. When an antioxidant is introduced to the ABTS+ solution, it reacts with the radical, causing a reduction in color intensity. As illustrated in Fig. 6, the antioxidant detection reagent containing the AgaA hydrolysis products exhibited a significant decolorization effect compared to the control group. This demonstrates that the NAOS generated from the AgaA-mediated hydrolysis of agarose possess significant antioxidant activity.
Fig. 6 Antioxidant activity analysis of AgaA hydrolysate.
Conclusion
The plasmid containing AgaA gene was successfully constructed and the active agarase was successfully expressed in E. coli Rosetta. The enzyme can effectively hydrolyze agarose to produce NAOS, and the product shows good antioxidant activity.
Reference
[1] Zhao, X., Li, X., He, L., Wang, L., & Zhang, Y. (2019). Production of neoagarobiose from agar through a dual-enzyme and two-stage hydrolysis strategy. Bioresource Technology, 278, 346-351. https://doi.org/10.1016/j.biortech.2019.01.06.