Part:BBa_K5093003

pET28a-EC.2.4.1.9

Sequence and Features

Construction Design

This engineered plasmid comprises a pET28a backbone (BBa_K3521004) and the gene EC 2.4.1.9 (BBa_K5093001).

Essential parts in the plasmid

EC 2.4.1.9 codes for the enzyme inulosucrase, which transfers a fructose group from the disaccharide sucrose to a growing inulin chain, a fiber, to produce glucose and inulin. The reaction is illustrated in Figure 3.

In our project, this enzyme reduces the absorption of glucose by catalyzing this reaction using sucrose as its substrate, hence lowering the chance of getting obese or contracting non-communicable diseases such as hyperglycemia, dyslipidemia, diabetes, coronary heart disease, non-alcoholic fatty liver disease, and stroke [1–15], without diminishing the sweetness of food and drink.

Its product, inulin, is a soluble dietary fiber that the gut microbiota can efficiently ferment. The high diversity of the gut microbiota has been proven to reduce the incidence of many chronic diseases, including inflammatory bowel disease, colorectal cancer, obesity, and T2DM [16–18]. Furthermore, dietary fiber could lower blood lipid concentration, reducing the risk of hyperlipidemia [18].

T7 Promoter (BBa_K3521002) and T7 Terminator (BBa_K3521002)

The T7 promoter and terminator originated in the T7 bacteriophage. The T7 promoter has a high affinity to its specific polymerase, the T7 RNA polymerase, which has a high transcription rate. When Isopropyl β-D-1-thiogalactopyranoside (IPTG), a lactose-like substance that bacteria cannot metabolize, is added, it binds to the Lac repressor on the operator to cause a conformation change, so the repressor is detached from the operator. T7 RNA polymerase can bind to the T7 promoter to initiate a fast transcription. This is very beneficial in the heterologous expression because the induction by IPTG can endure a high protein production rate.

Plasmid Backbone: pET28a (BBa_K3521004)

The pET28a plasmid has other desirable features that make it an ideal vector besides the T7 promoter and terminator it possesses. It has multiple restriction sites for the insertion of a new gene. Meanwhile, it has a sequence coding for a 6×histidine tag between the T7 promoter and terminator, so the protein produced can be purified via nickel column affinity chromatography. Another pronounced feature is the kanamycin resistance gene (KanR). When the target protein is made, this gene on the same plasmid is also expressed so that the bacteria containing the plasmid can survive under kanamycin. This essentially facilitates the preliminary selection of successfully transformed bacteria on kanamycin-containing media because the ones that fail to take in the plasmids are killed and unable to reproduce into clones.

Experimental Approach

1. Obtaining, Amplifying, and Identifying the Gene

The biotechnology company GeneScript synthesizes the DNA molecules containing our desired gene. Then, they are cut with restriction endonucleases NdeI and XhoI and amplified using polymerase chain reaction (PCR). The gene's length is 2400 bp. The bands representing EC 2.4.1.9 successfully appear at their corresponding positions in the gel, as shown in Figure 5, indicating that the cutting and amplifying are successful.

2. Plasmid Construction and Transformation

NdeI and XhoI are also used to cut pET28a to make complementary sticky ends. EC 2.4.1.9 is connected to the linear plasmids with T4 ligase. Then, the heat shock conversion of the recombinant plasmids is applied to competent E. coli DH5α. We then incubated them overnight at 37°C after streak inoculating them on LB solid medium plates that included appropriate antibiotics (LB-kana), as shown in Figure 6B.

Afterwards, we picked three colonies from each petri dish and extracted their plasmids. PCR and gel electrophoresis (shown in Figure 6A) were run to confirm the extracted plasmids were the ones we required. EC 2.4.1.9 (2400 bp long) appears at its corresponding position. Then, the pET28a-EC 2.4.1.9 plasmids are sent to Azenta Life Sciences for sequencing, whose results further proved our success in constructing the plasmid (Figure 7).

3. Protein Expression

The verified plasmids were transformed into E.coli BL21(DE3), incubated on LB solid medium plates (Kana+), and cultured at 37°C overnight. Four colonies were selected for PCR amplification to confirm success in the second transformation (Figure 8) and then transferred into 1L fresh LB (Kana+) culture medium for the scale-up cultivation.

IPTG (0.2 mM) was used to induce the expression of genes EC.2.4.1.9 with OD600 around 0.6-0.8 and cultured at 16°C for 20 hours. The proteins were then extracted from the supernatant of the E.coli BL21(DE3) after ultrasonic cell disruption and centrifugation. The size of inulosucrase is 88 kDa, as confirmed in the SDS-PAGE in Figure 9.

4. Protein Purification

Nickel affinity chromatography effectively purifies inulosucrase because the protein contains a 6×his tag. We obtained a more precise result with little interference from non-specifically bound proteins. Figure 9 shows only one band with a molecular weight of 88 kDa. This demonstrates that inulosucrase is successfully expressed and purified.

Other Test

We utilized thin-layer chromatography to verify that this enzyme can degrade sucrose. The principle of thin-layer chromatography is to use each component's different adsorption capacities on the same adsorbent so that the solvent flows through the adsorbent process, continuous adsorption, and desorption to achieve the mutual separation of the components. The reaction was carried out at 37°C for 1 hour in a buffer system with the addition of 2% plantain sugar and the appropriate amount of recombinant enzyme solution.

The results showed a reduction in sucrose and glucose production on the thin-layer chromatography plates when only 2% sucrose substrate was added, and the reaction was carried out at 37°C for 1 hour. This shows that this enzyme can break down sucrose to produce glucose and other substances in the reaction system.

In addition, sugarcane juice was used as a type of simulated food suspension to test enzyme function in real conditions. The experiment took place under 37°C to simulate human body temperature. A 1:1 ratio of concentration between dextransucrase and inulosucrase was used with masses of 1mg, 5mg, 10mg, 15mg, and 20mg of each type of enzyme per 100g sugarcane juice for 5 minutes, 10 minutes, 15 minutes, 30 minutes, and 60 minutes. Once the reaction time was reached, the solution was heated to 65°C to denature the enzymes.

Afterwards, HPLC was carried out to analyze the amount of sucrose and glucose in the solution. We used Origin Pro to process data, forming 3D mappings about glucose and sucrose concentrations in various conditions. By analyzing the raw data and the 3D mapping, we concluded that, in general, with a longer reaction time, catalyzing tends to become more complete, which means higher glucose concentration while lower sucrose concentration.

In speaking of each enzyme's sample size, except for the extremely high remaining sucrose with 1mg of dextransucrase and inulosucrase, it is difficult to summarize the overall effects of the change in glucose and sucrose concentrations. A low sucrose concentration (0g/100g) was left in the solution when 20mg of each enzyme was left and reacted for 60 minutes, but a higher glucose concentration was formed (2.9g/100g).

However, when the sample size is 10mg for each enzyme, noticeably low remaining sucrose (0.088g/100g) and relatively low glucose production (2.6g/100g) were observed when the reaction time was 15 minutes. In conclusion, we determined that allowing 10mg of each enzyme to react in sugarcane juice for 15 minutes is ideal to guarantee little sucrose sustain and promote glucose synthesis at 37°C.

References

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