New insights into the construction of wild-type Saba pig-derived Escherichia coli irp2 gene deletion strains

To construct wild-type E. coli irp2 gene deletion strains, CRISPR/Cas9 gene editing technology was used, and the difficulty and key points of gene editing of wild-type strains were analyzed. Based on the resistance of the CRISPR/Cas9 system expression vector, 4 strains of 41 E. coli strains isolated from Saba pigs were selected as the target strains for the deletion of the irp2 gene, which were sensitive to both ampicillin and kanamycin. Then, CRISPR/Cas9 technology was combined with homologous recombination technology to construct recombinant vectors containing Cas9, sgRNA and donor sequences to knock out the irp2 gene. Finally, the absence of the irp2 gene in E. coli was further verified by iron uptake assays, iron carrier production assays and growth curve measurements. The results showed that three of the selected strains showed single base mutations and deletions (Δirp2-1, Δirp2-2 and Δirp2-3). The deletion of the irp2 gene reduced the ability of E. coli to take up iron ions and produce iron carriers, but not affect the growth characteristics of E. coli. It is shown that the CRISPR/Cas9 knock-out system constructed in this study can successfully knock out the irp2 gene of the wild-type E. coli. Our results providing new insights into genome editing in wild-type strains, which enable further functional studies of the irp2 gene in wild-type E. coli.


Introduction
Saba pig is an excellent local breeding pig in Yunnan province in China, with wide distribution and large quantity, and is listed as a national livestock and poultry genetic resource protection breed (Lian et al. 2006). For a long time, due to inadequate feeding management and disease prevention and control, diarrhea and death caused by pathogenic E. coli infection in Saba pigs has become an important factor seriously threatening the development of characteristic pig industry in Yunnan province. The pathogenicity and virulence of E. coli are related to the high pathogenicity island (HPI), and the pathogenicity and virulence of E. coli are enhanced due to its existence (Rakin et al. 2013). Studies have shown that HPI has the characteristics of horizontal transfer, which has been found in different Enterobacteriaceae (Tu et al. 2017;Messerer et al. 2017;Benedek and Schubert 2007). HPI has a 30.5 kb functional core regions and carries irp1-irp9 genes related to iron element syntheses, regulation and uptake. Irp2 as a marker gene of HPI is an iron-regulated gene, which is only expressed in pathogenic Bo Zhang, Hongdan Wang, and Weiwei Zhao contributed equally to this work.
1 3 408 Page 2 of 9 bacteria and plays an important role in the syntheses of iron carriers and synthesis yersiniabactin (Ybt) (Tu et al. 2016;. Irp2 expresses the high molecular weight protein 2 (HMWP2), which is mainly involved in siderophore and induces the expression of ironophore. E. coli have the ability to acquire iron from host species, and this ability is a major influence factor on their pathogenesis. Some reports have shown that deletion of irp2 in E. coli abrogated Ybt production, reduced its ability to adhere to cells, and the LD50 value showed a reduction in its virulence (Smati et al. 2017;Tu et al. 2016). Therefore, it has potential values and significance to explore the relationship between iron uptake ability and irp2 gene in E. coli.
The CRISPR/Cas9 system composed of clustered regularly interspaced short palindromic repeats (CRISPR) and its affiliated Cas9 protein that exists on some bacteria and most archaic (Wiedenheft 2013). When foreign genes invade bacteria and archaic, they identify the invading DNA and insert it between the leader and repeat sequences of the CRISPR sequence, while the protospacer adjacent motif (PAM) to help Cas9 nuclease finds the cleavage site of the invading DNA, Cas9 protein then cleaves the foreign DNA to degrade it to protect the bacteria from harm (Hsieh-Feng and Yang 2020). Subsequently, the system was artificially modified with CRISPR/Cas9 gene editing technology (Demirci et al. 2018), which is simple, efficient and accurate compared to zinc finger nuclease (ZFN), transcriptional activator-like effector nuclease (TALENS) and homologous recombination technology (Urnov et al. 2010). It can be widely used in animals , plants Feng et al. 2013) and microorganisms (Cho et al. 2017) gene research. In CRISPR/Cas9 gene editing system, Cas9 protein is reflected on the double-strand break in DNA. If the broken gene is not repaired, the cell will die, which is one of the important factors that limit the effective function of the system. Most prokaryotic lack double-stranded DNA repaired system. When using CRISPR/Cas9 system to edit E. coli genes, the donor homologous to the target gene needs to be added to the vector as a template for repairing DNA double-strand breaks (DSB) to make sure that broke genes can be repaired. In addition, when homologous repair donor sequences exist, the double-stranded DNA cleaved by Cas9 protein can carry out spontaneous homologous recombination, and the repair efficiency is greatly improved (Altenbuchner 2016). Therefore, this work will adopt the strategy of combining CRISPR sgRNA and donor to knock out the irp2 gene of wild-type E. coli.
Although, the CRISPR/Cas9 technology has been widely and maturely applied in E. coli, there is still a paucity of reports on genome editing in wild-type E. coli, which would pose a problem for the study of wild-type E. coli gene functions. Therefore, this work intends to construct wild-type E. coli targeting the irp2 gene knockout through CRISPR/ Cas9 gene editing technology, and to explore the correlation between irp2 gene and iron uptake capacity of wild-type E. coli. Finally, the key points of using CRISPR/Cas9 technology to edit wild-type E. coli genes are highlighted, with a view to providing some reference for using this technology to edit the genomes of the remaining wild-type pathogens.

Materials
pEsgRNA-eGFP and pCas plasmids are relaxation plasmids, which are used in genome engineering ways. The pEsgRNA-eGFP plasmid (Biomics Biotech Company, Kunming, China) carries the ampicillin resistance gene (Ampicillin, 60 μg/ml). The plasmid pCas (Biomics Biotech Company, Kunming, China) carries kanamycin resistance gene (Kanamycin, 50 μg/ml) and can encode Cas9 nuclease. 41 wild-type E. coli strains were isolated and identified from a Saba swine farm in Chuxiong autonomous prefecture of Yunnan province in China. E. coli DH5α strain and CVCC1565 strain (irp2 + bacteria) were preserved in our laboratory. Bacterial genomic DNA extraction kit, agarose gel DNA recovery kit and plasmid mini-extraction kit were purchased from Tiangen Biochemical Technology Co. Ltd. (Kunming, China). Other reagents were all domestic analytical pure products.
Screening of irp2 gene knock-out target strains 41 E. coli strains isolated from Saba pigs were screened by LB medium containing ampicillin (60 μg/ml) and kanamycin (50 μg/ml) and the DNA of the selected strains was extracted by DNA extraction kit. The irp2 gene in wild-type E. coli was amplified by PCR using primers irp2-F: 5′-TTC CTT CAG TCG CCT GTT A-3′, irp2-R: 5′-CAA GCC CGA CAT ACT CAA TCT-3′ (GenBank No. BX-936398.1). Then, the PCR amplified products were identified by 1% agarose gel.

Construction of pEsgRNA-irp2 (T1, T2, and T3) plasmids
According to the design principle of sgRNA, the target site, upstream and downstream sequences of sgRNA were determined according to the results of irp2 gene sequence using online website (http:// spot. color ado. edu/ ~slin/ cas9. html). Then, 3 target locations were identified, named sgRNA-irp2T1, sgRNA-irp2T2, and sgRNA-irp2T3, respectively ( Table 1). The designed 3 pairs of sgRNA sequences were synthesized by the company and then connected.
After the pEsgRNA plasmid was extracted by kit, the pEsgRNA plasmid was digested with BamHI and XbaI restriction endonucleases to form the cohesive ends GATCC and CTAGA complementary to sgRNA. Then, 3 annealed double-stranded sgRNA (irp2T1, irp2T2, irp2T3) were linked with plasmid pEsgRNA which was digested by XbaI and BamHI restriction enzyme. Subsequently, the linked products were transformed into E. coli DH5α. After culture, 3 positive clones were selected from the plates transformed by pEsgRNA-sgRNA (irp2T1, irp2T2, and irp2T3) for sequencing verification. Finally, the correct vectors were named pEsgRNA-irp2T1, pEsgRNA-irp2T2, and pEsgRNA-irp2T3.

Construction of pEsgRNA-irp2 (T1, T2, and T3)-donor plasmids
To repair the irp2 gene effectively cut by Cas9 nuclease, the constructed pEsgRNA-irp2 (T1, T2, and T3) vectors need to inserted into the donor sequence which is homologous to the irp2 gene. Using irp2 gene as the template, the right and left donor primers were designed, and the irp2 gene was amplified by overlapping PCR. The primers information was shown in (Table 2).
The genomic DNA of the target strains were used as the template for the amplification of left and right donors. L-donor was amplified by primers L1 and L2, R-donor was amplified by primers R1 and R2. After acquiring L-donor and R-donor, connect them. The ligated donor and pEs-gRNA-irp2 (T1, T2, and T3) plasmids were treated with SalI and SphI endonuclease to produce the same cohesive ends. To connected donors with the pEsgRNA-irp2 (T1, T2, and T3) plasmids by T4-DNA ligase. All ligation products were transformed into E. coli DH5α, cultured overnight at 37 °C, then the positive clones were selected the next day. Subsequently, the donor sequence in the vector was amplified by PCR and verified by sequencing. Finally, the verified vectors were named pEsgRNA-irp2T1-donor, pEsgRNA-irp2T2-donor, and pEsgRNA-irp2T3-donor.

Irp2 gene knocking out by CRISPR/Cas9 gene editing
The pCas vector was transformed into target strains, and positive clones were screened by LB plate containing kanamycin. Subsequently, the constructed vectors pEsgRNA-irp2T1-donor, pEsgRNA-irp2T2-donor, and pEsgRNA-irp2T3-donor were transformed into the selected E. coli strains containing kanamycin resistance gene. There were four groups of each time-point (at 12, 24, 36, and 48 h). The first group included pCas and pEs-gRNA-irp2T1-donor, the second group included pCas and pEsgRNA-irp2T2-donor, the third group included pCas and pEsgRNA-irp2T3-donor, the last group included pCas, pEsgRNA-irp2T1-donor, pEsgRNA-irp2T2-donor, and pEsgRNA-irp2T3-donor. The positive clones were screened by LB plate containing ampicillin and kanamycin. Four positive clones of each group were chosen for PCR amplification and sequencing.  GATC GTC TCA GGA TTC GCT GTT ACC GTT TTA GAG  BamHI  CTAG CTC TAA AAC GGT AAC AGC GAA TCC TGA GAC  XbaI  sgRNA-irp2T2  GATC GAT TAC CAA CAA TTA CGC GAG GTT TTA GAG  BamHI  CTAG CTC TAA AAC CTC GCG TAA TTG TTG GTA ATC  XbaI  sgRNA-irp2T3 GATC GCC TTA CCC TTC GCG AGC TGT GTT TTA GAG BamHI CTAG CTC TAA AAC ACA GCT CGC GAA GGG TAA GGC XbaI

Determination of growth curves
After the target strains of E. coli were cultured overnight, then 200 μl culture solution was inoculated into 250 ml LB medium. The OD600 of culture was measured by ultraviolet spectrophotometer for periods of time ranging from 0 to 23 h. The growth curve of E. coli was plotted with time as abscissa and OD600 as ordinate.

Detection of iron carriers
The E. coli strains were inoculated into LBD liquid medium (2-2′-bipyridyl 0.4 mmol/l) for night culture, take 2 ml of the bacterial solution and centrifuged at 8000 r/min, then suck 1.5 ml of supernatant and add to the same volume of chrome azurol sulphonate (CAS) detection solution. When iron ions were dissociated from the CAS complex after 1 h, the color of the CAS blue detection solution became orange-yellow.
According to the ratio of the 630 nm light absorption of the CAS blue detection solution before and after the iron carrier was added, the concentration of test E. coli strains to produce iron carriers was determined (Schwyn and Neilands 1987). The ratio of A/Ar (Ar is the control value) as a quantitative indicator. The smaller the A/Ar ratio is, the larger the 1 − A/Ar ratio is, and the higher the yield of iron carriers is.

Determination of iron absorption capacity of E. coli strains
E. coli strains were infected with porcine intestinal epithelial cells (IPEC-J2 cells), and a control group was established at the same time. The cells and supernatant were collected at 3, 6, 9, 12, and 24 h. After centrifugation at 3000 rpm for 5 min, 200 μl supernatant was drawn after precipitation was removed, and the concentration of iron ion in cells was determined according to the instructions of iron determination kit. The significance of data difference was analyzed using GraphPad prism 6.0 and SPSS 24.0 software.

Screening of target strains and identification of irp2 gene
41 strains of wild-type E. coli were inoculated in LB medium containing ampicillin (Ampicillin concentration was 60 μg/ml), and 10 strains were sensitive to ampicillin. 10 strains of ampicillin sensitive E. coli were inoculated in LB medium (kanamycin concentration was 50 μg/ml), four strains of them were sensitive to ampicillin and kanamycin.
Finally, the irp2 gene was found in four strains of E. coli screened by PCR amplification, which could be used as irp2 gene knock-out target strains.

Construction of plasmids
Construction of pEsgRNA-irp2 (T1, T2, and T3) plasmids The pEsgRNA plasmid was linearized by double digestion with XbaI and BamHI enzymes. Then 3 sgRNAs were connected with the enzymatically digested pEsgRNA plasmid, whereafter the ligation products were transferred into E. coli DH5α, coated on a plate containing ampicillin and cultured overnight at 37 °C. The next day, 3 positive colonies were randomly selected from the plate to extract plasmids and sequenced, the sequence results were consistent with the original sgRNA sequence. The results showed that pEs-gRNA-irp2 (T1, T2, T3) plasmids were constructed.

Construction of pEsgRNA-irp2 (T1, T2, and T3)-donor plasmids
The overlapping PCR method was adopted to amplify left and right donors with primers L1, L2, R1, and R2. Then the left and right donors were linked. The ligated left and right donors were digesting and inserted into the vector pEsgRNA-irp2 (T1, T2, and T3) and transferred into E. coli DH5α. The positive clones were randomly selected from the resistant plate. PCR method was used to verify whether the donor was linked with pEsgRNA-irp2 (T1, T2, and T3) (Fig. 1a).

Construction of irp2 gene knock-out E. coli strains
The two irp2 gene editing vectors were co-electroporated into target strains. After electroporation, the positive clones were chosen by overnight culture on LB plate containing ampicillin and kanamycin. The positive clones were identified by PCR amplified and sequenced. The results indicated that the first group sequences remained. In the second group, point mutations of A → C and C → A as well as the deletion of C base were found at 1073, 1075, and 1076 of the irp2 gene sequences in pCas and pEsgRNA-irp2T2-donor plasmids transferred strains. In the third group of E. coli transferred by pCas and pEsgRNA-irp2T3-donor plasmids, point mutations of A → C, C → A, and C base deletion were observed at 1073, 1075, and 1076 of the irp2 gene sequence, respectively. C → A mutation and C base deletion occurred at 1075 and 1076 sites of irp2 gene sequence in the last group of E. coli transferred by pCas, pEsgRNA-irp2T1donor, pEsgRNA-irp2T2-donor, and pEsgRNA-irp2T3donor plasmids, respectively (Fig. 1b). Finally, four strains were named as 1R (wild-type strain), Δirp2-1, Δirp2-2, and Δirp2-3.

Determination of growth curves
Four strains of E. coli were inoculated into the liquid medium for oscillatory culture, and the optical density values of bacteria liquid were recorded in different time points. The growth curves of E. coli were drawn with the culture time as abscissa and optical density value of the bacterial liquid as the ordinate. The results showed that the growth trend of the strains before and after irp2 gene knockout was the same, especially in the delayed and stable periods (Fig. 1c).

The results of iron carrier medium detection
Four strains of E. coli and CVCC1565 strain were inoculated into the LBD iron-deficient medium. After overnight incubation, the supernatant was centrifuged and mixed with CAS blue detection liquid. After 1 h of rest, the light absorption value of the bacterial liquid was determined at 630 nm wavelength. The results showed that the 1 − A/Ar value (Ar value was 0.291) of strain CVCC1565 was the highest, and the ability to produce iron carriers were the highest. 1 − A/ Ar values of the other 3 strains were generally decreased (Table 3). It is suggested that the deletion of irp2 gene leads to a decrease in the ability of E.coli to produce iron carriers.

Effect of gene knock out on the uptake of iron by E. coli
The changes of iron in IPEC-J2 cells and supernatants were measured at 5 different time points using the iron ion detection kit after 4 strains of E. coli was infected with IPEC-J2. The results showed that the content of iron ion in the experimental group and the control group increased at first and then decreased. The content of iron ion in group 1R was less than that in group Δirp2. The content of iron in E. coli infection group was less than that in control group except at the 3rd hour. The content of iron in 1R group was significantly less than that in the control group at 5-time points (P < 0.01), and the content of iron Δirp2 group was lower than that in control group at 6th and 24th hour (P < 0.01), and less than in the control group at 9th hour (P < 0.05).
Besides, there was a significant difference in iron content of 1R group and Δirp2 group (P < 0.01), on the 3rd, 6th, and 9th hour (Fig. 2). The results showed that irp2 gene could mediate the iron absorption ability of E. coli, which was a great threat to cell growth.

Discussion
The CRISPR/Cas9 gene editing system mainly depends on vector resistance and the specificity of Cas9 nuclease expressed by sgRNA (Zerbini et al. 2017;Jiang et al. 2013). Because the vector carries resistance genes, positive clones can be screened from the resistance plate to decide whether the vector has been transferred to the target bacteria. It should be noted that in the gene editing of resistant strains, the selection of positive clones should fully consider the resistance genes carried by the selected vectors and the drug resistance of the strains. Therefore, from 41 wild-type E. coli screened 4 strains which were sensitive to Ampicillin and Kanamycin for gene editing. SgRNA is a special sequence with a length of about 20 bp and its 3′ end is close to the PAM sequence. It can complement and pair with the target site of genomic DNA as well as can also perform imperfect complementary pairing (off-target) with thousands of other sequences in the genome (Kleinstiver et al. 2015;Hsieh-Feng and Yang 2020). Therefore, when designing sgRNA of genomic target sites, we need to find PAM sequences in the Table 3 The quantitative detection of the iron load produced by E. coli The smaller the A/Ar ratio is, the larger the 1 − A/Ar ratio is, and the higher the yield of iron carrier is. The amount of iron carriers produced by E. coli CVCC1565 was the largest, and the amount of iron carriers produced by Δirp2 was lower than that of wild-type E. coli 1R  . 2 The changes of iron ion in IPEC-J2 cell and supernatant. P values were calculated using the Student's t test. P < 0.05(*) or P < 0.01(**) was considered statistically significant target DNA that can be recognized by Cas9. In addition, the designed sgRNA can be used for wild-type E. coli irp2 gene knockout, we need to obtain the irp2 gene sequence of the knock-out strains, and find the wild strains and E. coli engineered strains irp2 gene (the online addresses for sgRNA were designed using E. coli engineered bacterial genomes as templates) conserved region was used as template to design sgRNA. Finally, it is necessary to use software to check the specificity and potential off-target sites of gRNA.
In general, we should consider our experimental materials and experimental conditions, select the proper expression vector (plasmid), and the specificity of sgRNA to make the efficiency of gene editing. The editing of the target gene is of great significance to the study of its role. At present, genome editing technology based on CRISPR/Cas9 system is favored (Pyne et al. 2015;Sun et al. 2017), which has been applied to gene function research of zebrafish (Chang et al. 2013;Li et al. 2016), Arabidopsis , Saccharomyces cerevisiae (DiCarlo et al. 2013;Mans et al. 2015) and other organisms. CRISPR/Cas9 system produces double strands breaks (DSBs) in target genes by Cas9 nuclease, and then cells repair the damaged DNA through NHEJ or HDR pathway. NHEJ, as the main repair method of cells, can occur in any stage of the cell cycle. This repair method usually results in random insertion or deletion of several to hundreds of bases near the double-strand breaks, resulting in gene knockout (Hayashi and Tanaka 2019). In this research, three knock-out target sites were screened based on the irp2 gene sequence, one in the sense chain and the other two in the anti-sense chain. Three expression vectors were constructed according to three different gene knock-out target sites, then the expression vectors and pCas vector were transformed to the target strains. According to the sequencing results, there were base mutations and deletion in the designed sense chain target sites, indicating that one of the 3 vectors played a role and the other two expression vectors were out of the target. The reasons for off-target were related to the specificity of sgRNA, the concentration of Cas9-sgRNA, and the mismatch between DNA and RNA. In the process of gene editing by CRISPR/Cas9 gene editing technology, there will be off-target phenomenon. Therefore, we can select several more sites and choose sgRNA with high specificity when selecting target sites, the concentration of Cas9-sgRNA was optimized and a suitable expression vector was selected. At the same time, it may be necessary to consider the compatibility of the introduced exogenous expression plasmid with the endogenous plasmid of the target strain and whether the CRISPR/Cas9 system originally contained in the strain will affect the effect of the exogenous expression plasmid. For example, since Campylobacter jejuni contains the CRISPR/ Cas9 system, gene editing of this bacterium using CRISPR/ Cas9 gene editing technology requires the consideration of suppressing the activity of the Cas9 nuclease it contains to achieve the desired gene editing result. On the contrary, the CRISPR/Cas system in E. coli is type I-E, and the CRISPR/ Cas system of this type is inhibited by the DNA-binding protein H-NS (histone like nucleoid structure protein) when performing gene shearing function (Kiro et al. 2013). Therefore, when using CRISPR/Cas9 gene editing technology to edit E. coli genes, there is no need to consider the role of the CRISPR/Cas system. Only if all the above issues are fully considered and analyzed, then CRISPR/Cas9 gene editing technology will be more efficient when applied to gene editing of wild-type strains.
With the development of molecular biology technology, there have been many improvements in CRISPR/Cas9 technology. Jiang et al. (2015) introduced a homologous recombination system in Cas9 plasmid construction, while the donor sequence was later co-transferred into E. coli MG1655 with the expression plasmid to enable the CRISPR/Cas9 system to knock out several genes in this bacterium. The important improvement of this system is that the donor sequence does not need to be cloned inside the vector and is directly co-transformed with the plasmid, thus reducing the difficulty of the experiment. Wang et al. (2018) transferred pCas9 and pTargetF + donor plasmids into E.coli BL21, which not only achieved point mutation of the proB gene, but also avoid the risk of repeated cutting by gRNA/Cas9 without altering the PAM or inserting additional silent mutations into the genome. Li et al. (2021) modified the pCas/pTargetF system, CRISPR/Cas9 technology can be applied not only for gene editing of E. coli BL21(DE3), K-12 strains MG1655, DH5α, CGMCC3705 and other strains, but also to shorten the time to edit bacterial genomes. However, these studies were conducted on the genome of genetically engineered bacteria, not wild-type E. coli.
Existing online sgRNA design tools are not specifically targeted at wild-type E. coli. The evaluation of sgRNA off-target probability is based on E. coli K12, MG1655, BL21(DE3) instead of wild-type E. coli. It might lead to inaccurate evaluation of sgRNA off-target probability (Hou et al. 2020). So the sequences of wild-type E. coli irp2 gene need to be compared with those of E. coli using the online sgRNA design tool, and 3 sgRNA sequences were designed according to their conserved region sequences. In addition, given the different resistance phenotypes of wild-type E. coli, strains need to be screened for antibiotic sensitivity for gene editing. Therefore, 4 strains that were sensitive to both ampicillin and kanamycin were selected for gene knockout according to the resistance of the CRISPR/Cas9 system expression vectors. Finally, the irp2 gene was knocked out in three quarters of the wildtype E. coli strains with CRISPR/Cas9 technology combined with homologous recombination technology, which contained recombinant vectors with Cas9, sgRNA and donor sequences. From our current experimental results, the knock-out strategy can meet our requirements for gene editing of wild-type E. coli. In future research, it is still needed to expand the genome data of strains in the online sgRNA database, and modify the drug-resistant phenotype of wild-type strains according to the resistance of the expression vectors, so that the improved CRISPR/Cas9 system can be used for gene editing of more wild-type strains.
The irp2 gene is a marker gene of HPI, which is closely related to pathogenicity and virulence. As mentioned in the introduction, deletion of the irp2 gene results in the inability of the strain to synthesize Ybt and reduced virulence. Therefore, it has potential application values for the research of irp2 gene function. To explore the function of irp2 gene in wild-type E. coli, the Δirp2 strains were constructed by the CRISPR/Cas9 gene editing system, and the growth curves of the wild-type 1R and Δirp2 strains were measured. The growth curve showed that the delay, logarithm and stable phase of the 1R and Δirp2 strains were the same, indicating that irp2 gene is not the key gene for the growth of E. coli. The results of iron absorption test and quantitative detection of iron carrier production showed that irp2 gene could regulate the ability of E. coli to absorb iron and produce iron carrier, these results are of great significance for the research of the function of irp2 gene in E. coli. This work was the first to knock out the irp2 gene of E. coli from wild-type Saba pigs, which not only laid a foundation for the application of CRISPR/ Cas9 gene editing technology in microbial gene editing but also provided a certain reference basis for the study of irp2 gene function.