Published online Oct 15, 2003. doi: 10.3748/wjg.v9.i10.2240
Revised: May 25, 2003
Accepted: June 2, 2003
Published online: October 15, 2003
AIM: To clone flagellin genes A (flaA) and B (flaB) from a clinical strain of Helicobacter pylori (H pylori) and to construct prokaryotic expression systems of the genes and identify immunity of the fusion proteins.
METHODS: The flaA and flaB genes from a clinical H pylori isolate Y06 were amplified by high fidelity PCR. The nucleotide sequences of target DNA amplification fragments from the two genes were sequenced after T-A cloning. The recombinant expression vector pET32a inserted with flaA and flaB genes was constructed, respectively. The expressions of FlaA and FlaB fusion proteins in E. coli BL21DE3 induced by isopropylthio-β-D-galactoside (IPTG) at different concentrations were examined by SDS-PAGE. Western blot using commercial antibodies against whole cell of H pylori and immunodiffusion assay using self-prepared rabbit antiserum against FlaA (rFlaA) or FlaB (rFlaB) recombinant proteins were applied to the determination of the fusion proteins immunity. ELISA was used to detect the antibodies against rFlaA and rFlaB in sera of 125 H pylori infected patients and to examine rFlaA and rFlaB expression in 98 clinical isolates of H pylori, respectively.
RESULTS: In comparison with the reported corresponding sequences, the nucleotide sequence homologies of the cloned flaA and flaB genes were from 96.28%-97.13% and 96.31%-97.73%, and their putative amino acid sequence homologies were 99.61%-99.80% and 99.41%-100% for the two genes, respectively. The output of rFlaA and rFlaB expressed by pET32a-flaA-BL21DE3 and pET32a-flaB-BL21DE3 systems was as high as 40%-50% of the total bacterial proteins. Both rFlaA and rFlaB were able to combine with the commercial antibodies against whole cell of H pylori and to induce rabbits to produce specific antibodies with the same 1:2 immunodiffusion titers after the animals were immunized with the two recombinant proteins. Ninety-eight and zero point 4 and 92.80% of the serum samples from 125 patients infected with H pylori were positive for rFlaA and rFlaB antibodies, respectively. One hundred percent and 98.98% of the 98 tested isolates of H pylori were detectable for rFlaA and rFlaB epitopes, respectively.
CONCLUSION: Two prokaryotic expression systems with high efficiency of H pylori flaA and flaB genes were successfully established. The expressed rFlaA and rFlaB showed satisfactory immunoreactivity and antigenicity. High frequencies of FlaA and FlaB expression in different H pylori clinical strains and the general existence of specific antibodies against FlaA and FlaB in H pylori infected patients strongly indicate that FlaA and FlaB are excellent antigen candidates for developing H pylori vaccine.
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Citation: Yan J, Liang SH, Mao YF, Li LW, Li SP. Construction of expression systems for
flaA andflaB genes ofHelicobacter pylori and determination of immunoreactivity and antigenicity of recombinant proteins. World J Gastroenterol 2003; 9(10): 2240-2250 - URL: https://www.wjgnet.com/1007-9327/full/v9/i10/2240.htm
- DOI: https://dx.doi.org/10.3748/wjg.v9.i10.2240
In China, chronic gastritis and peptic ulceration are two most common gastric diseases, and gastric cancer is one of the malignant tumors with high mortalities and morbidities[1-34]. Helicobacter pylori (H pylori), a microaerophilic, spiral and Gram-negative bacterium, is considered as a human-specific gastric pathogen that colonizes the stomach of at least half of the world population[35]. Most infected individuals are asymptomatic. However, in some subjects, the infection causes acute, chronic gastritis and peptic ulceration, and plays important roles in the development of peptic ulcer and gastric adenocarcinoma, mucosa-associated lymphoid tissue (MALT) lymphoma and primary gastric non-Hodgkin’s lymphoma[36-43]. This microorganism has been categorized as class I carcinogen by the World Health Organization[44], and direct evidence of carcinogenesis has been recently demonstrated in animal models[45,46]. Immunization against the bacterium represents a cost-effective strategy to prevent H pylori-associated peptic ulcer diseases and to reduce the incidence of global gastric cancer[47]. Selection of antigenic targets is critical in design of H pylori vaccine. So far, no vaccine preventing H pylori infection has been commercially available. The majority of studies attempting to produce a vaccine have focused on urease enzyme, heat shock protein, and vacuolating cytotoxin[35,48-50], but rarely on H pylori flagellin. H pylori flagellin is composed of two subunits, named as FlaA with 53 KDa and FlaB with 54 KDa respectively. The flagellin plays a main role in motility and is necessary for colonization or persistence of H pylori infection[51]. The motility of H pylori is a virulent factor in the pathogenesis of gastric mucosal injury[52]. The data mentioned above indicate that FlaA as well as FlaB may be used as antigen candidates for H pylori vaccine. Therefore, in this study, two prokaryotic vectors responsible for expressing recombinant FlaA (rFlaA) and FlaB (rFlaB) were constructed . Immunoreactivity and antigenicity of rFlaA and rFlaB were further examined. Furthermore, these two recombinant proteins were used for detecting specific antibodies in sera from H pylori infected patients, and rabbit anti-rFlaA and anti-rFlaB sera were prepared for examining the corresponding epitopes of H pylori clinical isolates. The results of this study may contribute to the development of H pylori vaccines.
A clinical strain of H pylori was used in this study, which was provisionally named Y06, and well-characterized by the Department of Medical Microbiology and Parasitology, College of Medical Sciences, Zhejing University. A plasmid pET32a (Novagen) and an E. coli strain BL21DE3 (Novagen) were used as the expression vector and host cell, respectively. Primers for PCR amplification, the Pfu-Taq high fidelity PCR kit and restriction endonucleases were purchased from BioAsia (Shanghai, China). The T-A cloning kit and sequencing service were provided by BBST (Shanghai, China). Rabbit antiserum against the whole cell of H pylori, HRP-labeling sheep antisera against rabbit IgG and against human IgG were purchased from DAKO and Jackson ImmunoResearch, respectively. Agents used in isolation and identification of H pylori were purchased from Sigma and bioMérieux. Gastric biopsy specimens with positive H pylori isolation from 126 patients (86 males and 40 females, age range: from 6-78 years old, mean age: 40.5 years old) referred for gastroduodenoscopic examination in four different hospitals in Hangzhou were collected during the period between December 2001 and June 2002. Each of the patients gave a written informed content for this study. Of the 126 patients, 68 had chronic gastritis (CG, 48 superficial, 10 active and 10 atrophic), and the other 58 had peptic ulcer disease (PUD, 12 gastric ulcer, 40 duodenal ulcer and 6 gastric and duodenal ulcer). None of the patients had taken nonsteroidal anti-inflammatory drugs, antacids and antibiotics during the two weeks before seeking medical advice. At the same time, serum specimens were also collected from these patients.
Isolation and identification of H pylori Each gastric biopsy specimen was homogenized with a tissue grinder and then inoculated on Columbia agar plates supplemented with 8.0% (V/V) sheep blood, 0.5% (W/V) cyclodextrin, 5 mg/L trimethoprim, 10 mg/L vancomycin, 2500 U/L cefsoludin and 2.5 mg/L amphotericin B. The plates were incubated at 37 °C under microaerobic conditions (5% O2, 10% CO2 and 85% N2) for 3 to 5 d. A bacterial isolate was identified as H pylori according to typical Gram staining morphology, biochemical tests positive for urease and oxidase, and agglutination with the commercial rabbit antibody against whole cell of the microbe. All of H pylori isolates were stored at -70 °C for ELISA.
Preparation of DNA template Genomic DNA of H pylori strain Y06 was extracted by the conventional phenol-chloroform method and DNase-free RNase treatment[52]. The obtained DNA was dissolved in TE buffer, and its concentration and purity were determined by ultraviolet spectrophotometry[52].
Polymerase chain reaction Oligonucleotide primers were designed to amplify the whole sequence of flaA and flaB genes from H pylori strain Y06 based on the published corresponding genomic sequences[53-56]. The sequence of flaA sense primer with an endonuclease site of EcoRV was 5’-CCGGATATCATGGCTTTTCAGGTCAA-3’. The sequence of flaA antisense primer with an endonuclease site of XhoI was 5’-CCGCTCGAGAAACTAAGTTAAAAGCC-3’. The sequence of flaB sense primer with an endonuclease site of EcoRI was 5’-CCGGAATTCATGAGTTTTAGGATAAA-3’. The sequence of flaB antisense primer with an endonuclease site of XhoI was 5’-CCGCTCGAGCTGTTATTGTAAAA GCC-3’. The total volume per PCR was 100 µL containing 2.5 mol·L-1 each dNTP, 500 nmol·L-1 each of the two primers, 15 mol·L-1 MgCl2, 3.0 U Pfu-Taq polymerase, 100 ng DNA template and 1 × PCR buffer (pH8.8). The parameters for PCR were at 94 °C for 5 min, × 1; at 94 °C for 30 s, at 52 °C for 30 s, at 72 °C for 90 s, × 10; at 94 °C for 30 s, at 52 °C for 30 s, at 72 °C for 100 s (10 s addition for the each of the following cycles), × 15; then at 72 °C for 10 min, × 1. The results of PCR were observed under UV light after electrophoresis in 15 g·L-1 agarose pre-stained with ethidium bromide. The expected sizes of target amplification fragments were 1530 bp for flaA gene and 1542 bp for flaB gene.
Cloning and sequencing The target amplification DNA fragments from flaA and flaB genes were respectively cloned into pUCm-T vectors (pUCm-T-flaA and pUCm-T-flaB) by using the T-A cloning kit according to the manufacturer’s instructions. The recombinant plasmids were amplified in an E. coli strain DH5α and then extracted by the Sambrook’s method[57]. A professional company (BBST) was responsible for nucleotide sequence analysis of the inserted fragments. Three strains of E. coli DH5α containing pUCm-T-flaA, pUCm-T-flaB and expression vector pET32a were amplified in BL medium, and the three plasmids were extracted, respectively[57]. These plasmids were digested with EcoRV and XhoI, EcoRI and XhoI, respectively. The flaA target fragment and pET32a, and the flaB fragment and pET32a were recovered and then ligased. The recombinant expression vectors pET32a-flaA and pET32a-flaB were respectively transformed into E.coli BL21DE3, and the expression systems were named as pET32a-flaA-BL21DE3 and pET32a-flaB-BL21DE3. The target fragments of flaA and flaB genes inserted in pET32a plasmid were sequenced again.
Expression and identification of fusion proteinspET32a-flaA-BL21DE3 and pET32a-flaB-BL21DE3 were rotatively cultured in LB medium at 37 °C induced by isopropylthio-β-D-galactoside (IPTG) at different concentrations of 1.0, 0.5 and 0.1 mmol·L-1. The supernatant and precipitate were separated through centrifugation after the bacterial pallet was ultrasonically broken (300 V, 5 s × 3). The molecular weight and output of rFlaA and rFlaB were examined by SDS-PAGE. The two recombinant proteins were collected by Ni-NTA affinity chromatography. The commercial rabbit antiserum against whole cell of H pylori and HRP-labeling sheep antiserum against rabbit IgG were used as the first and second antibodies to determine the immunoreactivity of rFlaA and rFlaB by Western blot. Rabbits were immunized with rFlaA and rFlaB, respectively, for preparation of antisera. Immunodiffusion assay was applied to the determination of the antigenicity of rFlaA and rFlaB.
ELISA The specific antibodies against FlaA and FlaB in sera of the 126 patients infected with H pylori were detected by ELISA, by using rFlaA and rFlaB as antigens at the coated concentration of 20 µg/mL and a patient serum sample (1:400 dilution) as the first antibody and HRP-labeling sheep antibody against human IgG (1:4000 dilution) as the second antibody. The result of ELISA for a patient’s serum sample was considered as positive if the optical density at 490 nm (OD490) was over the mean plus 3 SD of five negative serum samples[58]. FlaA and FlaB expression in clinical isolates of H pylori was detected by ELISA using the ultrasonic supernatant of each H pylori isolate (50 µg/mL) as a coated antigen, the self-prepared rabbit antisera against rFlaA and rFlaB (1:800 dilution in both) as the first antibody and HRP-labeling sheep antibody against rabbit IgG (1:3000 dilution) as the second antibody. The result of ELISA for a H pylori ultrasonic supernatant sample was considered as positive if its OD490 value was over the mean plus 3 SD of five ultrasonic supernatant samples at the same protein concentration of E. coli ATCC 25922[58].
Date analysis The nucleotide sequences of the cloned flaA and flaB genes were compared for homology with the 3 published flaA gene sequences (NC000915, NC000921, X60746)[53-55] and the 4 published flaB gene sequences (NC000915, NC000921, L08907, AF479024)[53,54,56,59] by using a molecular biological analysis software.
Target fragments of flaA and flaB genes with expected sizes amplified from DNA template of H pylori stain Y06 are shown in Figure 1.
The nucleotide sequences of flaA gene in pUCm-T-flaA and pET32a-flaA were completely the same and so as for flaB gene. The homologies of nucleotide and putative amino acid sequences of the cloned flaA gene compared with the published flaA sequences[53-55] were from 96.28% to 97.13% and from 99.61% to 99.80%, respectively (Figure 2 and Figure 3). The homologies of nucleotide and putative amino acid sequences of the cloned flaB gene were 96.31%-97.73% and 99.41%-100%, compared with the published flaB sequences (Figure 4 and Figure 5)[53,54,56,59].
IPTG at concentrations of 1.0, 0.5 and 0.1 mmol·L-1 efficiently induced the expression of rFlaA and rFlaB in pET32a-flaA-BL21DE3 and pET32a-flaB-BL21DE3 systems. The products of rFlaA and rFlaB were mainly presented in ultrasonic precipitates, and the output was 40%-50% of the total bacterial proteins (Figure 6 and Figure 7).
The commercial rabbit antibodies against the whole cell of H pylori combined with rFlaA and rFlaB as confirmed by Western blot (Figure 8 and Figure 9). Both the titer of immunodiffusion assay between rFlaA and its rabbit antiserum, rFlaB and its rabbit antiserum was 1:2.
Since the mean ± SD of OD490 values of the five negative serum samples were 0.338 ± 0.036 for rFlaA and 0.102 ± 0.051 for rFlaB in the detection of specific antibodies in patients’ sera, the positive reference value was 0.446 for FlaA and 0.255 for FlaB. According to the reference values, 98.4% (123/125, one serum sample was contaminated) of the tested patients’ serum samples were positive for antibodies against rFlaA with an OD490 value range of 0.52-1.76, and 92.8% (116/125) were positive for antibodies against rFlaB with an OD490 value range of 0.26-1.50. Since the mean ± SD of OD490 of the five negative bacterial controls was 0.200 ± 0.046 for FlaA and 0.170 ± 0.044 for FlaB in the detection of clinical H pylori isolates, the positive reference value was 0.338 for FlaA and 0.302 for FlaB. According to the reference values, 100% (98/98) of the tested H pylori isolates were detectable for the epitope of rFlaA with an OD490 value range of 0.36-2.01 and 99% (97/98) of the isolates were detectable for the epitope of rFlaB with an OD490 value range of 0.31-1.78.
In the present study, H pylori flaA and flaB genes were detected in genomic DNA of almost all H pylori isolates, and their nucleotide and amino acid sequences were considerably conserved[53,54]. The FlaA and FlaB expressed by H pylori rendered the organism strong motility in mucous environment, induced IL-8 secretion and facilitated inflammation in gastric tissue[51,52]. Furthermore, we observed that serum antibodies against FlaA and FlaB were present in approximate 98.4% and 92.8% of H pylori infected patients, respectively, the rates were significantly higher than those of heat shock protein (68%) and vacuolating cytotoxin (68%)[60]. These data indicate that flaA and flaB genes express their products in majority of H pylori strains and efficiently induce specific antibodies, implying a brilliant potential for developing H pylori vaccine.
The flaA gene from H pylori strain Y06, cloned in this study, showed high homologies of nucleotide and putative amino acid sequences compared with the published corresponding sequences (Figure 2 and Figure 3)[53-55]. Similarly, the homologies of nucleotide and putative amino acid sequences of the cloned flaB gene from H pylori strain Y06 were quite high when compared with the published corresponding sequences (Figure 4 and Figure 5)[53,54,56-59]. The high conservation of nucleotide and putative amino acid sequences found in the cloned flaA and flaB genes were probably due to their expression products just as the structural peptides of H pylori.
In the present study, SDS-PAGE demonstrated that the constructed expression systems pET32a-flaA-BL21DE3 and pET32a-flaB-BL21DE3 were able to efficiently produce the target recombinant proteins. However, rFlaA and rFlaB were mainly presented with the form of inclusion body even if they were induced by IPTG at a lower concentration. The high output of rFlaA and rFlaB (40%-50%) was beneficial to the production of a possible H pylori vaccine.
The rabbit antiserum against the whole cell of H pylori recognizes and combined with rFlaA and rFlaB as confirmed by Western blot, indicated that the two recombinant proteins had a relatively high immunoreactivity. The immunodiffusion assay performed in this study demonstrated that rFlaA and rFlaB could efficiently induce rabbit to produce specific antibodies with a higher titer, which indicated that these two recombinant proteins exhibited favorable antigenicity.
All tested H pylori isolates (98/98) expressed FlaA while 99.0% (97/98) of the tested isolates expressed FlaB, as detected by ELISA. Of the H pylori infected patients, 98.4% (123/125) and 92.8% (116/125) were seropositive for the specific antibodies against rFlaA and against rFlaB, respectively. The universal existence of FlaA and FlaB in H pylori strains and the efficient induction of specific antibodies against FlaA and FlaB in patients were the strong favorable evidences for using these two recombinant proteins as the potential antigens in the development of H pylori vaccine.
In conclusion, FlaA and FlaB are excellent and ideal antigens that can be potentially used for the development of H pylori vaccine, and the expression systems of FlaA and FlaB with a high efficiency has been successfully constructed.
We are grateful to the four hospitals in Hangzhou that provided gastric biopsies in this study, which help us to complete the research subject.
Edited by Xia HHX and Wang XL
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