Development of a CRISPR/Cas9 genome editing toolbox for Corynebacterium glutamicum

Background

Corynebacterium glutamicum is an important industrial workhorse and advanced genetic engineering tools are urgently demanded. Recently, the clustered regularly interspaced short palindromic repeats (CRISPR) and their CRISPR-associated proteins (Cas) have revolutionized the field of genome engineering. The CRISPR/Cas9 system that utilizes NGG as protospacer adjacent motif (PAM) and has good targeting specificity can be developed into a powerful tool for efficient and precise genome editing of C. glutamicum.

Results

Herein, we developed a versatile CRISPR/Cas9 genome editing toolbox for C. glutamicum. Cas9 and gRNA expression cassettes were reconstituted to combat Cas9 toxicity and facilitate effective termination of gRNA transcription. Co-transformation of Cas9 and gRNA expression plasmids was exploited to overcome high-frequency mutation of cas9, allowing not only highly efficient gene deletion and insertion with plasmid-borne editing templates (efficiencies up to 60.0 and 62.5%, respectively) but also simple and time-saving operation. Furthermore, CRISPR/Cas9-mediated ssDNA recombineering was developed to precisely introduce small modifications and single-nucleotide changes into the genome of C. glutamicum with efficiencies over 80.0%. Notably, double-locus editing was also achieved in C. glutamicum. This toolbox works well in several C. glutamicum strains including the widely-used strains ATCC 13032 and ATCC 13869.

Conclusions

In this study, we developed a CRISPR/Cas9 toolbox that could facilitate markerless gene deletion, gene insertion, precise base editing, and double-locus editing in C. glutamicum. The CRISPR/Cas9 toolbox holds promise for accelerating the engineering of C. glutamicum and advancing its application in the production of biochemicals and biofuels.

The Gram-positive soil bacterium Corynebacterium glutamicum was discovered about 60 years ago, and was originally well-known as an excellent producer of glutamate [1]. With the development of biotechnology, C. glutamicum has been successfully engineered to serve as a versatile workhorse for industrial bioproduction. Nowadays, this bacterium is used to produce more than 4 million tons of diverse amino acids per year and a wide range of other natural and non-natural products, which are used as feed additives, nutritional supplements, pharmaceutical intermediates, biofuels, and polymer building blocks [2]. It is estimated that products generated via C. glutamicum fermentation will reach a market size of US$20.4 billion by 2020 [3].

At the early stage of engineering of C. glutamicum, random mutagenesis combined with positive selection by phenotypic resistance to amino acid analogs was the most commonly used strategy [4]. Genetic manipulations in C. glutamicum were initiated in 1984 and became a key enabling strategy for strain improvement [5]. A routinely used method for gene disruption and insertion in C. glutamicum is based on integration of a suicide vector into its chromosome, followed by a second recombination event to remove the plasmid backbone and a counter-selection step using a conditionally lethal marker. Nevertheless, due to the frequent spontaneous inactivation of the counter-selectable marker sacB, up to 45% of colonies obtained in the screening process were false-positive, making this multi-step procedure time-consuming and inefficient [6].

Recently, clustered regularly interspaced short palindromic repeats (CRISPR) and their CRISPR-associated proteins (Cas) have been explored as a leading-edge tool for genome editing in eukaryotic host cells, plants, and animal models of human disease [7,8,9]. Although CRISPR/Cas systems (especially CRISPR/Cas9 systems) are derived from bacteria or archaea, their applications have not been extensively employed in bacteria [10]. To date, successes of bacterial genome editing using CRISPR/Cas9 systems have been reported in limited bacteria including Escherichia coli [11,12,13,14,15,16,17,18,19], Streptococcus species [11, 20], Lactobacillus reuteri [21], Streptomyces species [22,23,24], Tatumella citrea [12], Clostridium species [25,26,27,28,29], Bacillus subtilis [30,31,32], Myceliophthora species [33], and Synechococcus elongates [34].

To engineer C. glutamicum more efficiently and unleash its potential in industrial biotechnology, facile yet robust genome editing tools are urgently demanded. The CRISPR/Cas9 system that utilized NGG as protospacer adjacent motif (PAM) and has good targeting specificity is expected to enable genome-wide scale and precise editing of GC-rich C. glutamicum [10]. To our knowledge, there were many tries in the community to adapt CRISPR/Cas9 into C. glutamicum for comprehensive genome editing. In the time this manuscript was being prepared, Cho and coworkers reported CRISPR/Cas9-mediated genome editing of C. glutamicum using cas9 gene codon-optimized for its use in actinomycetes and recT gene encoding E. coli prophage recombinase [35]. Without the use of recT, no positive transformants could be obtained using double-stranded DNA (in both linear and replicative plasmid form) or single-strand DNA (ssDNA) as editing templates. Further introduction of recT facilitated deletion of 400-bp chromosomal fragments using ssDNA as editing templates. However, Cho and coworkers didn’t report whether the optimized CRISPR/Cas9 system including RecT could delete or insert genes into the chromosome of C. glutamicum with plasmid-borne templates [35]. Meanwhile, Jiang and coworkers independently developed a CRISPR/Cpf1-mediated genome editing tool for C. glutamicum [36]. The CRISPR-Cpf1 system combined with ssDNA recombineering can efficiently introduce small changes into the C. glutamicum genome. Large gene deletions and insertions are also realizable using this system [36]. However, because Francisella novicida Cpf1 utilizes a T-rich PAM [37], its editing targets in GC-rich C. glutamicum genome are supposed to be fewer than Streptococcus pyogenes Cas9. Therefore, development of a powerful CRISPR/Cas9-mediated genome editing toolbox that can delete, insert and modify genes in C. glutamicum flexibly and multiply is still urgently demanded.

In this study, we successfully developed a CRISPR/Cas9 toolbox for efficient and comprehensive engineering of several C. glutamicum strains. By using the tailor-made CRISPR/Cas9 system, gene deletion and insertion with plasmid-borne editing templates were achieved with efficiencies of 30.8–60.0% and 16.7–62.5%, respectively. CRISPR/Cas9-mediated ssDNA recombineering was developed to introduce small modifications and single-nucleotide changes into the genome with efficiencies over 80.0%. Double-locus editing was also realized in C. glutamicum with an efficiency of 40.0%. The toolbox developed here is simple and versatile, which will provide solutions to overcome major limitations of existing genome editing technologies of C. glutamicum and advance engineering and application of this industrial workhorse.

Optimization of Cas9 and gRNA expression for lethality-based selection

It has been repeatedly reported that the double-strand breakage (DSB) induced by Cas9 is lethal to bacterial cells because many microorganisms lack the endogenous nonhomologous end joining (NHEJ) mechanism, or the NHEJ is not efficient enough to repair the DSB. As a result, CRISPR/Cas9 was usually used as a lethality-based selection tool in bacterial cells [25, 26]. To achieve CRISPR/Cas9-mediated genome editing, the lethality of Cas9-induced DSB was first evaluated.

Constitutive expression of dCas9 from S. pyogenes in C. glutamicum has been proven unattainable [3]. In a previous study, isopropyl-β-d-thiogalactopyranoside (IPTG)-inducible promoter P _tac and propionate-inducible promoter P _prpD2 were used for dCas9 expression, and P _tac was used for gRNA expression, facilitating CRISPR interference (CRISPRi) in C. glutamicum [3]. Inspired by this study, we used the same biological parts to prepare Cas9 and gRNA expression cassettes. Strictly controlled expression of Cas9 was considered beneficial for screening desirable mutants when using CRISPR/Cas9 for gene deletion [26]. To optimize the promoter for Cas9 expression, P _tac and P _prpD2 were employed to drive the expression of a Cas9-red fluorescent protein (RFP) fusion protein that consisted of the first 180 bp of cas9 gene and the full-length rfp gene. The artificial P _tac /P _prpD2 -cas9 ^180bp-rfp cassettes were inserted into pXMJ19, generating plasmids pRfp1 and pRfp2, respectively (Fig. 1a). Fluorescence outputs of the engineering cells harboring pRfp1 and pRfp2 were detected in the presence or absence of inducers. The results demonstrated that P _tac was controlled more strictly by IPTG than P _prpD2 by sodium propionate (Fig. 1b). Plasmid pCas9 was then constructed by inserting P _tac -cas9 cassette into pXMJ19 and transformed into C. glutamicum SL4, a derivative of strain ATCC 13869 with high electrotransformation efficiency, generating strain SL4 (pCas9). The gRNA targeting on the C. glutamicum lactate dehydrogenase gene ldhA was designed and inserted into pEC-XK99E under the control of P _tac , resulting in pgRNA1. Transformation of pgRNA1 into strain SL4 (pCas9) was performed and cells were spread on soya peptone-glucose-yeast extract (SGY) plates containing kanamycin (Km) and chloramphenicol (Cm) with or without 1 mM IPTG. All the colonies growing on the plates were counted to calculate the escape rate. A high escape rate (8.7 ± 1.9 × 10⁻²) was obtained, which was unacceptable for lethality-based selection.

Optimization of CRISPR/Cas9 system in C. glutamicum. a Schematic representation of the plasmids used for optimizing the promoter of Cas9 expression. The cas9 ^180bp-rfp fusion gene that consisted of the first 180 bp of cas9 gene and the full-length rfp gene was inserted into pXMJ19 under the control of IPTG-inducible promoter P _tac (pRfp1) or propionate-inducible promoter P _prpD2 (pRfp2). The empty plasmid pXMJ19 was used as a negative control. b Optimization of promoters for Cas9 expression. pRfp1, pRfp2, and pXMJ19 were transformed into C. glutamicum SL4 separately. The resultant transformants were cultivated in SGY medium with or without 1 mM IPTG (for pRfp1) or 1 g/L sodium propionate (for pRfp2). Cells of the stationary growth phase were used to detect their fluorescence outputs using a microplate reader (λ excitation = 560 nm, λ emission = 607 nm). c Schematic representation of the plasmids used for verifying the function of the terminator derived from S. pyogenes (T _Sp ). A rfp gene was inserted downstream the gRNA (pRfp3) and the modified gRNA with T _Sp deleted (pRfp4). The empty plasmid pEC-XK99E was used as a negative control. d Function verification of T _Sp in E. coli and C. glutamicum by detecting fluorescence outputs of strains harboring pRfp3, pRfp4, or pEC-XK99E. e The gRNA structure derived from plasmid pgRNA1. f The optimized gRNA structure derived from plasmid pgRNA2. g Escape rate of CRISPR/Cas9-based counter-selection using different gRNA expression plasmid. pgRNA1 and pgRNA2 were transformed into C. glutamicum SL4 (pCas9) separately. Correct transformants were cultivated, diluted and spread on SGY plates containing Km and Cm, with or without IPTG (1 mM). The escape rate of counter-selection was calculated by colony counting

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The unoptimized gRNA expression cassette may be one reason for the high escape rate of CRISPR/Cas9-based counter-selection. Considering that cas9 and gRNA were both under control of P _tac , P _11F which is a derivative of the strong constitutive promoter P _cspB of C. glutamicum [38] was recruited for gRNA expression to avoid possible interference between the two P _tac promoters. The secondary structure of gRNA is also crucial for forming Cas9-gRNA complex. The gRNA used here consists of three domains: a 20–25 nt complementary region for specific DNA binding, a 42 nt hairpin for Cas9 binding (Cas9 handle), and a 40 nt transcription terminator derived from S. pyogenes (T _Sp ) [39]. T _Sp functioned well in E. coli and many other bacteria [26, 30, 39]. It was also recruited to develop CRISPRi in C. glutamicum, but its termination ability has not been investigated in C. glutamicum [3]. To evaluate T _Sp , a rfp gene was inserted into the downstream of gRNA, producing plasmid pRfp3. T _Sp of pRfp3 was further deleted, resulting in plasmid pRfp4 (Fig. 1c). As expected, deletion of T _Sp increased rfp expression in E. coli, demonstrating that T _Sp was functional in E. coli. However, the rfp downstream T _Sp was highly expressed in C. glutamicum and deletion of T _Sp decreased rfp expression (Fig. 1d). This surprising phenomenon suggests that T _Sp does not function as a terminator in C. glutamicum. In plasmid pgRNA1, T _Sp was followed by a 185 bp redundant segment and a rrnB terminator (T _rrnB ). Since T _Sp could not terminate gRNA transcription in C. glutamicum, the 185 bp redundant segment will also be transcribed, which may affect the function of Cas9-gRNA complex (Fig. 1e). To confirm our hypothesis, the 185 bp redundant segment was removed from plasmid pgRNA1. The resultant plasmid pgRNA2 harbored a gRNA expression cassette in which T _rrnB closely followed T _Sp (Fig. 1f). Lethality test using pCas9 and pgRNA2 showed that the escape rate was reduced to 1.3 ± 0.2 × 10⁻², making the CRISPR/Cas9-based counter-selection feasible (Fig. 1g).

Markerless chromosomal gene deletion using CRISPR/Cas9 and plasmid-borne editing template

Since the CRISPR/Cas9 system could act as an efficient selection tool, we exploited its capacity for markerless chromosomal gene deletion. Two ~ 1000 bp homologous arms flanking at both sides of the targeted ldhA gene were inserted into plasmid pgRNA2. The resultant plasmid pgRNA3 was then transformed into C. glutamicum SL4 (pCas9) to provide a DNA editing template for deleting 664 bp of ldhA gene. It was expected that edited mutants would be generated through double-crossover homologous recombination and nonedited cells would be eliminated by CRISPR/Cas9-directed cleavage at the targeted ldhA gene (Fig. 2a). Noteworthily, the transformants obtained could be divided into two categories, abnormally large ones and small ones (Fig. 2b). Colony PCR was conducted to confirm gene deletion in the transformants using a pair of primers shown in Fig. 2a. All the abnormally large colonies were false and two of the twenty small ones tested were positive mutant (Additional file 1: Figure S1).

Gene deletion using CRISPR/Cas9 and plasmid-borne editing template in C. glutamicum SL4. a Schematic representation of pCas9, pgRNA3, and gene deletion event. b Transformants harboring pCas9 and pgRNA3 on a SGY plate supplemented with Km, Cm, and IPTG (1 mM). pCas9 and pgRNA3 were co-transformed into strain SL4 simultaneously and cells were spread on SGY plates with Km, Cm, and IPTG (1 mM) immediately after recovery. Colonies marked in red cycles were the so-called abnormally large colonies. c Schematic representation of different patterns of pCas9 mutation. Gene deletion, cas9 gene was removed from pCas9. Nonsense mutation, a T465G mutation occurred, generating a stop codon (TAT to TAG) in cas9 gene. Insertional inactivation, a transposase encoding gene from E. coli was inserted into cas9 gene, which deactivated cas9. d Colony counting and editing efficiency calculation of C. glutamicum SL4. Colonies on SGY plates supplemented with Km, Cm, and IPTG (1 mM) were counted and verified using colony PCR. e PCR verification of ldhA deletion in C. glutamicum SL4 using the primer pair (ldhA-up and ldhA-down) shown in a. M, DNA marker; –, wild-type control; 1–8, eight small colonies. This displayed the result of Replicate 1 in c. The results of Replicate 2 and Replicate 3 were shown in Additional file 1: Figure S2

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Although successful gene deletion was achieved by using CRISPR/Cas9 system, the editing efficiency was quite low. We speculated that two events might help the false positives escape the counter-selection. First, the targeted DNA was cleaved by Cas9 but the DSB was repaired by nucleotide or base excision repair, leading to the survival of cells and very likely some mutations at the cleavage site [40]. In this case, the targeted gene might be deactivated but PCR was not capable of verifying it. Second, pCas9 or pgRNA3 mutated, which disabled the Cas9-gRNA complex and the counter-selection system. To confirm our hypotheses, the ldhA genes of false positives were amplified by PCR and sequenced. pCas9 and pgRNA3 were also extracted from the false positives and sequenced. No mutation was found in gene ldhA or plasmid pgRNA3, whereas plasmid pCas9 mutated in several patterns as shown in Fig. 2c. In all the abnormally large colonies investigated, their cas9 genes were all deleted from pCas9 plasmids. In the small but false colonies, their cas9 genes were either deactivated through nonsense mutation or disrupted by insertion of a transposase encoding gene from E. coli. Such cells harboring mutated pCas9 escaped the counter-selection, and even worse, outgrew those expressing active Cas9, making selection of the edited cells very difficult.

Since cas9 was easily mutated in C. glutamicum, reducing replication of pCas9 in the host may lessen the mutation. A one-step electrotransformation strategy was then presented that pCas9 and pgRNA3 were co-transformed into C. glutamicum SL4 simultaneously and cells were spread on SGY plates supplemented with Km, Cm, and IPTG (1 mM) immediately after recovery. Screening using two antibiotics and expressing cas9 may burden cell growth, and colonies appeared after 2–3 days cultivation. We still got some abnormally large colonies and they were all proven false by colony PCR. However, the ratio of positive mutants out of all colonies obtained in one plate considerably increased, reaching an average of 47.3 ± 11.9% (Fig. 2d, e; Additional file 1: Figure S2). Given the high editing efficiency, edited cells should be easily obtained after CRISPR/Cas9 counter-selection. Meanwhile, a control experiment was conducted using pCas9 and pgRNA3-derivative plasmid that harbored no targeting spacer. As expected, no counter-selection phenomenon was observed and no gene deletion mutants were obtained (Additional file 1: Figure S3).

Markerless chromosomal gene insertion

Next, the ability of gene insertion (allelic exchange) by using CRISPR/Cas9 system was examined. A rfp cassette (781 bp) was inserted between the upstream and downstream homologous arms of pgRNA3. The resultant plasmid pgRNA4, together with pCas9, was co-transformed into C. glutamicum SL4, aiming to replace the ldhA gene with the rfp cassette (Δ664 bp and insert 781 bp) (Fig. 3a). Colony PCR was conducted to verify the gene insertion events by using a pair of primers shown in Fig. 3a. An average of 25.0 ± 8.3% of colonies were confirmed as positive mutants (Fig. 3b, c; Additional file 1: Figure S4). The mutant inserted with the rfp cassette in the ldhA gene was designated as C. glutamicum SL4ΔldhA::rfp.

Gene insertion using CRISPR/Cas9 and plasmid-borne editing template in C. glutamicum SL4. a Schematic representation of pCas9, pgRNA4, and gene insertion event. b Colony counting and editing efficiency calculation of C. glutamicum SL4. pCas9 and pgRNA4 were co-transformed into C. glutamicum SL4 simultaneously and cells were spread on SGY plates supplemented with Km, Cm, and IPTG (1 mM) immediately after recovery. Colonies on the selective plates were counted and verified using colony PCR. c PCR verification of rfp insertion in C. glutamicum SL4 using the primer pair (rfp-up and ldhA-down) shown in a. M, DNA marker; –, wild-type control; 1–10, ten small colonies. This displayed the result of Replicate 1 in b. The results of Replicate 2 and Replicate 3 were shown in Additional file 1: Figure S4

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ssDNA-directed recombineering using CRISPR/Cas9 and RecT

ssDNA-directed recombineering can be used to mutagenize, repair or engineer the chromosome with high efficiencies [41]. By introducing exogenous recombinases into C. glutamicum, the recombination efficiency using ssDNA templates was much higher than that using plasmid-borne templates [42]. However, due to lack of reliable genotype selection method, application of this technique was severely limited. Taking advantage of the CRISPR/Cas9 system developed here, counterselecting mutants generated during recombineering against wild-type cells became feasible and a ssDNA-directed gene editing tool was developed. The recT gene encoding recombinase RecT of prophage Rac was inserted into plasmid pgRNA4 under the control of the propionate-inducible promoter P _prpD2 , resulting in plasmid pgRNA5 (Fig. 4a). ssDNAs were designed to alter the PAM sequence or PAM-proximal 8–12 bp sequences because these regions were shown to be most crucial for Cas9 targeting specificity [43]. To obtain high recombination efficiency, 90mer ssDNAs targeted to the lagging strand were used here.

ssDNA-directed recombineering using CRISPR/Cas9 and RecT in C. glutamicum SL4ΔldhA::rfp. a Schematic representation of pCas9 and pgRNA5 which were used for ssDNA-directed recombineering. b Operation scheme of ssDNA-directed recombineering using CRISPR/Cas9 and RecT for rfp deactivation. A 90mer ssDNA targeted to the lagging strand (rfp-off1, Additional file 1: Table S1) is designed to introduce two successive stop codons (highlighted in red) in rfp gene. PAM sequence of the gRNA is shaded grey. Plasmid pgRNA5 was first transformed into C. glutamicum SL4ΔldhA::rfp. The resultant strain SL4ΔldhA::rfp (pgRNA5) was cultivated in SGY medium supplemented with Km and sodium propionate to induce RecT expression. Electrocompetent cells were then prepared and transformed with pCas9 and ssDNA. After recovery, cells were spread on SGY plates supplemented with Km, Cm, and IPTG (1 mM) to induce Cas9 expression for counter-selection. Colonies were picked randomly and verified by measuring their fluorescence outputs. c Fluorescence output detection of candidate mutants of C. glutamicum SL4ΔldhA::rfp ^off1. –, wild-type C. glutamicum SL4 control; +, C. glutamicum SL4ΔldhA::rfp; 1–10, ten colonies. This displayed the result of Replicate 1. The results of Replicate 2 and Replicate 3 were shown in Additional file 1: Figure S6. d rfp gene sequencing of C. glutamicum SL4ΔldhA::rfp ^off1 mutants. Nucleotides in red box represents the two successive stop codons (TAG TAA) introduced by ssDNA-directed recombineering. e Str^R phenotype test of C. glutamicum SL4 rpsL ^K43R mutants. Ten colonies were picked randomly from SGY plates supplemented with Km, Cm, and IPTG (1 mM) and patched onto SGY plates (Str⁻) and SGY plates supplemented with streptomycin (Str⁺). Seven out of ten colonies were Str^R. f rpsL gene sequencing of C. glutamicum SL4 rpsL ^K43R mutants. Nucleotides in red box represents the mutated codon (AAG to CGC) introduced by ssDNA-directed recombineering

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The method was first tested for the ability to introduce stop codons into a target gene. A ssDNA (rfp-off1, Additional file 1: Table S1) was designed to introduce two successive stop codons into the rfp gene of C. glutamicum SL4ΔldhA::rfp (Fig. 4b). The operation scheme was shown in Fig. 4b. Plasmid pgRNA5 was first transformed into strain SL4ΔldhA::rfp. The resultant strain SL4ΔldhA::rfp (pgRNA5) was cultivated with addition of sodium propionate to induce RecT expression, and then electrocompetent cells were prepared. Next, cells were co-transformed with pCas9 and ssDNA, recovered, and spread on SGY plates supplemented with Km, Cm, and IPTG (1 mM) to induce Cas9 expression. Three independent experiments were conducted and hundreds of colonies could be obtained in each experiment, which were much more than the number of colonies got in gene deletion and insertion experiments (Additional file 1: Figure S5). For each replicate, 10 colonies were picked randomly and verified by measuring their fluorescence outputs, (Fig. 4c; Additional file 1: Figure S6). The gene editing events were further verified by gene sequencing (Fig. 4d), demonstrating a high editing efficiency of 86.7 ± 5.8%, an average of 90.0, 90.0, and 80.0% from three replicates. Such high mutation rate would eliminate the need of phenotype screening methods for ssDNA-directed recombineering, making genome editing of C. glutamicum more efficient.

Ribosomal protein S12 encoding gene rpsL was selected as another target for ssDNA-directed gene editing using CRISPR/Cas9. An amino acid mutation K43R (AAG to CGC in the nucleotide sequence) resulting in resistance to streptomycin (Str^R) was described for C. glutamicum [44, 45]. A ssDNA was designed to mutate AAG to CGC which corresponded to amino acid mutation K43R, and plasmid pgRNA6 was then constructed. Using the protocol described previously, mutants with Str^R phenotype were obtained with a mutant efficiency of 70.0% (Fig. 4e). Gene sequencing further verified the targeted gene editing of rpsL (Fig. 4f).

Plasmid curing

To cure the Cas9 and gRNA expression plasmids for continuous genome editing, engineered cells were cultivated in SGY medium without antibiotics for 12 h. The culture was serially transferred into fresh medium for another two times before plating on SGY plates without antibiotics. The resultant colonies were picked and tested for resistance to Km and Cm. Approximately 25.0% of colonies were sensitive to Km and Cm, confirming that both plasmids were cured. In the study that reported CRISPR/Cpf1-mediated genome editing of C. glutamicum, Jiang et al. replaced the replicon of pXMJ19 (cas9 expression plasmid) with a temperature sensitive replicon pBL1^ts [46] and deleted the distribution protein Per encoding gene [47] in pEC-XK99E (gRNA expression plasmid), facilitating easy plasmid curing [36]. Since plasmids with the same backbones were used in our and Jiang et al.’s studies [36], the strategy reported by Jiang et al. is also applicable to optimizing the present plasmid curing procedure.

CRISPR/Cas9-mediated genome editing in C. glutamicum wild-type strains

To evaluate the universality of the CRISPR/Cas9-mediated genome editing toolbox described above, its application was tested in two well-known wild-type C. glutamicum strains ATCC 13869 and ATCC 13032. ldhA gene knockout was first performed. After co-transformation of pCas9 and pgRNA3, cells were spread on SGY plates supplemented with Km, Cm, and 1 mM IPTG. However, the cell growth was severely hindered. Colonies of strain ATCC 13869 appeared after 8 days cultivation and no colonies of strain ATCC 13032 were obtained even after 10 days cultivation. Considering that expression of Cas9 can be a significant burden for cell growth, we hypothesized that the expression level of Cas9 was too high for strains ATCC 13969 and ATCC 13032. Therefore, the inducer (IPTG) usage was reduced and 0.1 mM IPTG and 0.01 mM IPTG were proven suitable for strains ATCC 13969 and ATCC 13032, respectively. After 2–3 days cultivation, colonies were picked for verification, revealing that ldhA deletion efficiencies reached 33.3 ± 2.5 and 60.0% in strains ATCC 13969 and ATCC 13032, respectively (Table 1). When shorter homologous arms (~ 500 bp) were used to knock out ldhA in strain ATCC 13032, fewer colonies but comparable deletion efficiency (50.0%) were obtained (Table 1), indicating that shorter homology arms may result in lower homologous recombination efficiencies. An 8083 bp fragment (cgl1776–cgl1781) was selected as a second target for CRISPR/Cas9-mediated gene deletion in strain ATCC 13032. Using plasmids pCas9 and pgRNA9 harboring ~ 1000 bp homologous arms, the 8083 bp fragment was successfully deleted with an efficiency of 40.0% (Table 1).

By using plasmids pCas9 and pgRNA4, replacement of ldhA gene with the rfp cassette was conducted in strains ATCC 13969 and ATCC 13032. The editing efficiencies reached 28.6 and 62.5%, respectively (Table 1). Then, in order to assess the possibility of inserting larger DNA fragments into the genome of C. glutamicum using CRISPR/Cas9, we attempted to insert a 3626 bp lacZ cassette into the genomic locus between cgl0900 and cgl0901 without deleting any chromosomal fragment. By co-transforming pCas9 and pgRNA10 into strain ATCC 13032, insertion of the lacZ cassette was achieved at an efficiency of 50.0% (Table 1). These results demonstrate the possibility of deleting and inserting larger DNA fragments in C. glutamicum.

By using pCas9, pgRNA5 and ssDNA rfp-off1 (Additional file 1: Table S1), ssDNA-directed recombineering was also successfully performed in C. glutamicum ATCC 13032::rfp with an editing efficiency of 90.0% (Additional file 1: Figure S7). The achievable genome editing of different C. glutamicum strains with slight modification of inducer usage suggests a possible broader applicability of the CRISPR/Cas9-mediated genome editing toolbox.

Single-nucleotide editing

Adaptive evolution and mutagenesis breeding usually generate hundreds of single nucleotide polymorphisms (SNPs) in the genome sequence. Single-nucleotide editing is a key enabling strategy to investigate the function of SNPs and assemble positive mutations (SNPs) to construct hyper producing strains. To explore the application of CRISPR/Cas9 system in single-nucleotide editing, a ssDNA (rfp-off2, Additional file 1: Table S1) was designed to change C to G in rfp gene (three bases upstream of the PAM sequence), which generated a stop codon. Similar editing efficiency (90.0%) was obtained (Additional file 1: Figure S8), demonstrating that the CRISPR/Cas9 system could be applied to precise base editing.

Double-locus editing

Since ssDNA-directed recombineering achieved considerably high editing efficiency of single-locus editing, we then doubled the number of editing targets. rfp and rpsL were selected as targets for double-locus editing and pgRNA7 that possessed two gRNA expression cassettes targeting rfp and rpsL were constructed (Fig. 5a). When C. glutamicum ATCC 13032::rfp harboring pgRNA7 was co-transformed with pCas9 and two kinds of ssDNAs (rfp-off1 and rpsL-K43R, Additional file 1: Table S1), only ten colonies were obtained, which were much fewer than those obtained in single-locus editing. All the ten colonies were verified and four of them were the expected double-mutants, demonstrating a double-locus editing efficiency of 40.0% (Fig. 5b). With the number of editing loci increased, the number of colonies obtained decreased dramatically. Therefore, simultaneous editing of more than two loci is still difficult to achieve. It is speculated that higher recombination efficiency would be helpful.

Double-locus editing in in C. glutamicum. a Schematic representation of pCas9 and pgRNA7 which were used for ssDNA-directed recombineering. b Mutants verification by sequencing of rfp and rpsL genes. Plasmid pgRNA7 that simultaneously expressed two gRNAs targeting rfp and rpsL was first transformed into C. glutamicum ATCC 13032::rfp. The resultant strain was then induced to express RecT and co-transformed with pCas9 and two kinds of synthetic ssDNAs (10 μg rfp-off1 and 10 μg rpsL-K43R, Additional file 1: Table S1). After recovery, cells were spread on SGY plates supplemented with Km, Cm, and IPTG (0.01 mM) to induce Cas9 expression for counter-selection. Colonies were picked and verified by gene sequencing

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As a gram-positive bacterium with good genomic stability, C. glutamicum is more difficult to engineer than genetically tractable hosts such as E. coli [40, 48]. CRISPR/Cas9-mediated ssDNA recombineering was developed for deleting 400 bp chromosomal fragment in C. glutamicum in the time this manuscript was being prepared [35]. However, gene deletion and insertion with plasmid-borne editing templates that are key enabling techniques for reconstruction and integration of metabolic pathways are still in demand. In this study, a tailor-made CRISPR/Cas9 toolbox was developed for efficient and comprehensive engineering of C. glutamicum. Notably, gene deletion and insertion with plasmid-borne editing templates were efficiently implemented. Moreover, single-nucleotide editing and double-locus editing were achieved at efficiencies of 90.0 and 40.0%, respectively, which will considerably accelerate precise genome editing of C. glutamicum.

S. pyogenes Cas9 is suggested to be toxic to C. glutamicum and difficult to be introduced into C. glutamicum [35, 36]. As an alternative, F. novicida CRISPR/Cpf1 system was recruited to perform genetic manipulation of C. glutamicum recently [36]. Compared to the CRIPSR/Cpf1 tool, the present CRISPR/Cas9 tool has some distinct advantages. First, the efficiencies of CRISPR/Cas9-mediated gene deletion and insertion using plasmid-borne editing templates were higher than those obtained by CRIPSR/Cpf1. Second, the CRISPR/Cas9 system is more suitable for genome-wide scale engineering of C. glutamicum. Because Cpf1 utilizes a T-rich PAM and Cas9 utilizes NGG as PAM [36, 37, 49], Cas9 has considerably more editing targets in C. glutamicum. A bioinformatics analysis of the genome sequence of C. glutamicum ATCC 13032 revealed 332,289 Cas9 targets in coding sequences, which is 169.6% of the number of Cpf1 targets (195,978) (Additional file 2: Table S2). Third, Cas9 possesses better targeting specificity and can be used for precise editing, including single-nucleotide editing. Since Cpf1 cannot distinguish a single-nucleotide mismatch in seed sequence, additional synonymous mutations need to be introduced near the targeting position [36, 37]. However, even a single synonymous mutation may alter the secondary structure of the mRNA and the expression of the mutant protein [50], limiting application of the CRIPSR/Cpf1 tool in precise editing.

Considering the advantages of CRISPR/Cas9 system, attempts to introduce the S. pyogenes cas9 gene with native codon into C. glutamicum were made but failed, which may be attributable to its strong expression and non-specific binding to the chromosomal DNAs [35, 36]. To reduce the translation efficiency, the cas9 gene originally codon-optimized for atinomycetal genomes was recruited [35]. However, in this study, the cas9 gene with native codon was successfully transformed into C. glutamicum and used for counter-selection. The same IPTG-inducible promoter P _tac but different ribosome binding sites from the previous studies were used here, which may lead to successful introduction of the cas9 gene. The previous and present results all suggest that fine-tuning of Cas9 expression is crucial for application of CRISPR/Cas9 system in bacteria. Another unexpected crucial factor was discovered that the frequently used gRNA terminator derived from S. pyogenes (T _Sp ) did not terminate transcription in C. glutamicum. As a consequence, redundant RNA segments would be transcribed with the gRNA, which might affect the function of Cas9-gRNA complex. Deletion of the 185 bp redundant segment between T _Sp and plasmid-borne T _rrnB resulted in an acceptable escape rate (1.3 ± 0.2 × 10⁻²) for counter-selection.

During CRISPR/Cas9-mediated microbial genome editing progress, production of false positives seemed inevitable even in E. coli, of which the escape rate of counter-selection was quite low [11, 12, 16]. CRISPR/Cpf1-assisted editing also suffers from the same problems [36]. Although such false positives will disturb screening of edited cells, the mechanism behind the phenomenon remained unclear [16]. Here we demonstrated that modification on the cas9 gene was the main cause of producing such false positives (Fig. 2c). In the case of CRISPR/Cpf1-assisted editing, Cpf1 mutations may also be the major reason for false positives formation since editing efficiency decreased when continuous editing was conducted using the Cpf1 expression plasmid transformed in the former round of editing [36]. By using a one-step electrotransformation strategy to reduce replication of pCas9 in the host, we alleviated the problem and increased gene deletion efficiency significantly. Previous studies suggested that small amount of Cas9 proteins produced by leaky expression can already lead to introduction of DSB resulting in SOS induction [51]. Our experiments also showed that even in the absence of gRNA, Cas9 expression hindered cell growth of C. glutamicum. Therefore, we hypothesized that such SOS induction in C. glutamicum may lead to modification of the cas9 expression cassette. To overcome this obstacle, more strictly controlled promoter is needed for Cas9 and Cpf1 expression.

Electrotransformation and homologous recombination efficiencies of C. glutamicum are another two key factors that affects the acquisition of edited mutants [35]. In this study, C. glutamicum SL4, a derivative of strain ATCC 13869, was first selected as the target strain because of its high electrotransformation efficiency. Comparative genome analysis between strains SL4 and ATCC 13869 revealed some mutations in cell wall synthesis-related genes, such as flippase, arabinosyltransferase, and murein biosynthesis protein encoding genes. It is speculated that these mutations may contribute to the high electroporation efficiency of strain SL4 and further studies on the mechanism are underway. In some cases (e.g., gene deletion in C. beijerinckii), serial subculturing was applied to compensate for the low homologous recombination efficiency and enrich edited cells [26]. However, because false positives would outgrow edited cells, such strategy was unsuitable for the present case. Previous studies demonstrated that introducing exogenous recombinase or exonuclease benefited homologous recombination in C. glutamicum [35, 42, 52], which gave us inspiration to improve the editing efficiency of the CRISPR/Cas9 toolbox.

In summary, a CRISPR/Cas9 toolbox was developed for efficient and comprehensive engineering of the industrial workhorse C. glutamicum. Markerless gene deletion, gene insertion, single-nucleotide editing and double-locus editing were achieved by using a customized two-plasmid-based CRISPR/Cas9 system and a simplified co-transformation strategy. This toolbox works well in several C. glutamicum strains and holds promise for renovating the genome editing of corynebacteria.

Microorganisms, cultivation conditions, and plasmids

All bacterial strains used in this study are listed in Table 2. E. coli DH5α was used for general cloning and cultivated aerobically at 37 °C in Luria–Bertani (LB) broth. Km (25 μg/mL) or Cm (20 μg/mL) was added to LB broth as required. C. glutamicum ATCC 13869 and C. glutamicum ATCC 13032 were obtained from the American Type Culture Collection (ATCC). C. glutamicum SL4 was a derivative of strain ATCC 13869 with high electrotransformation efficiency. C. glutamicum SL4 and its derivatives were cultivated aerobically at 30 °C in SGY medium containing 18 g/L soya peptone, 5 g/L glucose, 10 g/L yeast extract, 1 g/L K₂HPO₄·3H₂O, 1 g/L urea, 0.5 g/L succinic acid, and 10 μg/L biotin. C. glutamicum ATCC 13032, C. glutamicum ATCC 13869 and their derivatives were cultivated aerobically at 30 °C in SGY medium or LBHIS medium [53]. Km (25 μg/mL), Cm (5 μg/mL), streptomycin (Str, 25 μg/mL) or IPTG (0.01 to 1 mM) was added in the medium as required. All plasmids used in this study (Table 2) were constructed using ClonExpress II One Step Cloning Kit or ClonExpress MultiS One Step Cloning Kit (Vazyme, Nanjing, China), which facilitated ligation of two or more DNA fragments through 15–20 bp overlaps. Primers and synthetic ssDNAs used for genetic manipulation are listed in Additional file 1: Table S1.

Electrotransformation protocol of C. glutamicum

C. glutamicum SL4 and its derivatives cultivated overnight in SGY medium were inoculated into 100 mL fresh SGY medium to an OD_600nm value of 0.3. When OD_600nm value reached ~ 0.8, cells were collected by centrifugation at 8000 rpm and 4 °C for 10 min. After washed with ice-cold deionized distilled water for 4 times, cells were resuspended in 0.5 mL 10.0% (v/v) glycerol and 100 μL aliquots of competent cells were obtained. DNA (less than 10 μL) was added to the competence cells and transferred to a 2 mm electroporation cuvette (BioRad) with parameters set at 2500 V and 5 ms. Electroporations were performed with Eppendorf Electroporator 2510. After electroporation, 1 mL SGY medium was added immediately. Cells were incubated for 2–6 h at 30 °C, and spread on SGY plates supplemented with antibiotics and IPTG as required. The plates were incubated at 30 °C until colonies appeared. Regarding to C. glutamicum ATCC 13869, C. glutamicum ATCC 13032 and their derivatives, preparation of competent cells and electrotransformation were performed according to the protocols described previously [53].

Construction of Cas9 and gRNA expression plasmids and determination of Cas9-induced lethality

To optimize the promoter for Cas9 expression, plasmids pRfp1 and pRfp2 were constructed. The first 180 bp of cas9 gene and the full-length rfp gene were amplified by PCR from pRed_Cas9_recA_Δpoxb300 [54] and pEC-XK99E-rfp using primer pairs cas9 ^180bp-1/cas9 ^180bp-2 and rfp-1/rfp-2, respectively. The cas9 ^180bp segment and rfp gene were subcloned into the HindIII and PstI sites of pXMJ19 under control of P _tac , producing pRfp1. P _prpD2 , cas9 ^180bp, rfp, and pXMJ19 backbone were amplified by PCR using primer pairs P _prpD2 -1/P _prpD2 -2, cas9 ^180bp-3/cas9 ^180bp-4, rfp-1/rfp-2, and pXMJ19-1/pXMJ19-2, respectively, and assembled into pRfp2. pRfp1 and pRfp2 were introduced into C. glutamicum SL4 through electrotransformation separately. The transformants were cultivated in the presence or absence of 1 mM IPTG (for pRfp1) or 1 g/L sodium propionate (for pRfp2). Cells of the stationary growth phase were used to detect their fluorescence outputs using a microplate reader (λ excitation = 560 nm, λ emission = 607 nm).

To construct plasmid pCas9, the cas9 gene was amplified by PCR using primer pair cas9-1/cas9-2 from pRed_Cas9_recA_Δpoxb300 [54] and inserted into the HindIII and PstI sites of pXMJ19 under control of P _tac . Plasmid pgRNA1 was produced by ligating lacIq-P _tac fragment, gRNA fragment targeting ldhA and pEC-XK99E backbone. The three DNA fragments were amplified by PCR from pXMJ19, pRed_Cas9_recA_Δpoxb300 and pEC-XK99E using primer pairs P _tac -1/P _tac -2, gRNA-3/gRNA-4 and pEC-XK99E-4/pEC-XK99E-5, respectively. The gRNA targeting ldhA contained a base-pairing region (N24 5′-GTGGATATCCTGACCTACGCAGTG-3′), a Cas9 handle and a S. pyogenes terminator (T _sp ). In plasmid pgRNA1, the rrnB terminator (T _rrnB ) from pEC-XK99E backbone located in the185 bp downstream of T _sp .

In order to confirm whether T _sp can work in C. glutamicum, plasmids pRfp3 and pRfp4 were constructed. pRfp3 was a derivative of pEC-XK99E carrying the gRNA (targeting ldhA) and rfp gene driven by the constitutive promoter P _11F . P _11F -gRNA was amplified by PCR from pgRNA1 using primer pair gRNA-1/gRNA-2. The rfp gene was amplified by PCR from pEC-XK99E-rfp using primer pair rfp-4/rfp-5, and the pEC-XK99E backbone was amplified using primer pair pEC-XK99E-1/pEC-XK99E-2. To construct pRfp4, the backbone of pRfp3 was amplified by PCR to remove the T _sp and rfp gene using primer pair pEC-XK99E-3/pEC-XK99E-1. The rfp gene was amplified by PCR from pRfp3 using primer pair rfp-5/rfp-6 and ligated to the backbone of pRfp3, resulting in pRfp4. pRfp3 and pRfp4 were introduced into E. coli MG1655 and C. glutamicum SL4 through electrotransformation separately. Cells of the stationary growth phase were used to detect their fluorescence outputs using a microplate reader (λ excitation = 560 nm, λ emission = 607 nm).

Plasmid pgRNA2 was derived from pgRNA1 by replacing P _tac with P _11F and deleting the 185 bp region between T _sp and T _rrnB . The P _11F -gRNA fragment was amplified by PCR from pgRNA1 using primer pair gRNA-1/gRNA-6. pgRNA1 backbone was amplified by PCR using primer pair pEC-XK99E-6/pEC-XK99E-2 to remove the 185 bp region. The two fragments were ligated to form pgRNA2.

To determine the escape rate of counter-selection, 1 μg pCas9 was transformed into C. glutamicum SL4. Cells were spread on SGY plates supplemented with Cm after 2 h recovery. After cultivated at 30 °C for 2 days, colonies were picked and verified by colony PCR. The correct transformant was designated as C. glutamicum SL4 (pCas9). Then pgRNA1 and pgRNA2 were transformed into C. glutamicum SL4 (pCas9) separately. Correct transformants were cultivated, diluted and spread on SGY plates containing Km and Cm, with or without IPTG (1 mM). The escape rate of counter-selection was calculated by colony counting.

Gene deletion and insertion using CRISPR/Cas9

To provide editing template for ldhA deletion, two homologous arms of ldhA (~ 1 kb for each arm) were amplified by PCR from the genomic DNA of C. glutamicum SL4 using primer pairs ldhA-1/ldhA-2 and ldhA-3/ldhA-4, respectively. The backbone of pgRNA2 was amplified by PCR using primer pair pEC-XK99E-8/pEC-XK99E-9. pgRNA3 was constructed by ligating the two homologous arms and pgRNA2 backbone. Plasmid pgRNA4 was derived from pgRNA3 by inserting a rfp cassette between the two homologous arms of ldhA. The rfp cassette and pgRNA3 backbone were amplified by PCR using primer pairs rfp-7/rfp-8 and ldhA-2/ldhA-5, respectively. The two fragments were ligated to form pgRNA4. Plasmid pgRNA8 was derived from pgRNA3 by replacing the ~ 1 kb homologous arms with ~ 500 bp homologous arms for ldhA deletion. Primer pairs ldhA-6/ldhA-7 and pEC-XK99E-8/pEC-XK99E-9 were used to amplify the homologous arms and plasmid backbone from plasmid pgRNA3. The two fragments were ligated to form pgRNA8. Plasmid pgRNA9 was constructed to delete the cgl1776-cgl1781 fragment (8083 bp). Primer pairs pEC-XK99E-13/pEC-XK99E-8 and pEC-XK99E-9/pEC-XK99E-14 were used to amplify two plasmid backbone fragments from plasmid pgRNA3. Primer pairs 8083-1/8083-2 and 8083-3/8083-4 were used to amplify two homologous arm fragments from the genomic DNA of C. glutamicum ATCC 13032. The four fragments were ligated to form pgRNA9. Plasmid pgRNA10 was constructed to insert the lacZ cassette (3626 bp) into the genomic locus between cgl0900 and cgl0901 in C. glutamicum ATCC 13032. Primer pairs pEC-XK99E-15/pEC-XK99E-8 and pEC-XK99E-9/pEC-XK99E-16 were used to amplify two plasmid backbone fragments from plasmid pgRNA3. Primer pairs 3626-1/3626-2 and 3626-3/3626-4 were used to amplify two homologous arm fragments from the genomic DNA of C. glutamicum ATCC 13032. Primer pair lacZ-1/lacZ-2 was used to amplify the lacZ cassette from the genomic DNA of E. coli MG1655. The five fragments were ligated to form pgRNA10.

Regarding to ldhA deletion in C. glutamicum SL4, 1 μg pgRNA3 was transformed into C. glutamicum SL4 (pCas9). Cells were recovered at 30 °C for 6 h and then spread on SGY plates supplemented with Km, Cm, and IPTG (1 mM). Plates were incubated at 30 °C for 2–3 days until colonies appeared. The C. glutamicum SL4ΔldhA mutants were verified by colony PCR using primer pair ldhA-up/ldhA-down. PCR products of edited cells were 1604 bp, and those of wild-type cells were 2268 bp. When the one-step electrotransformation strategy was used, 3 μg pCas9 and 1 μg pgRNA3 were co-transformed into C. glutamicum SL4. Mutants screening and verification were performed using procedures described above. Regarding to rfp insertion in C. glutamicum SL4, the one-step electrotransformation strategy described above was used except that pCas9 and pgRNA4 were co-transformed into C. glutamicum SL4 and primer pair rfp-up/ldhA-down was used for PCR verification of C. glutamicum SL4ΔldhA::rfp mutants. PCR products of edited cells were 1449 bp.

For gene deletion and insertion in C. glutamicum ATCC 13869 and ATCC 13032, pCas9 and pgRNA3 (pgRNA4, pgRNA8, pgRNA9, or pgRNA10) were co-transformed. After electroporation, 1 mL LBHIS broth was added immediately and the suspension was quickly incubated for 6 min at 46 °C [53]. Cells were then incubated for 6 h at 30 °C and subsequently spread on SGY or LBHIS plates supplemented with Km, Cm, and IPTG (0.01 or 0.1 mM), Plates were incubated at 30 °C for 2–3 days until colonies appeared. Mutants verification were performed by colony PCR using the primer pairs shown in Additional file 1: Table S1.

CRISPR/Cas9-mediated ssDNA recombineering

Plasmid pgRNA5 was construct by inserting a P _prpD2 -recT cassette into pgRNA2 and replacing the base-pairing region of gRNA targeting ldhA with a base-pairing region targeting rfp (N20, 5′-GCGGTCTGGGTACCTTCGTA-3′). A part of pgRNA2 backbone was amplified by PCR using primer pair gRNA-7/pEC-XK99E-8. N20 for rfp was added to the backbone by primer gRNA-7. A second part of pgRNA2 backbone was amplified by PCR using primer pair pEC-XK99E-9/pEC-XK99E-10. P _prpD2 and recT were amplified by PCR using primer pairs P _prpD2 -3/P _prpD2 -4 from the genomic DNA of C. glutamicum ATCC 13032 and recT-1/recT-2 from the genomic DNA of E. coli MG1655, respectively. The four fragments were ligated to form the pgRNA5. To construct plasmid pgRNA6, the backbone of pgRNA5 was amplified by PCR using primer pair pEC-XK99E-11/pEC-XK99E-12 with replacement of the base-pairing region of gRNA targeting rfp with a base-pairing region targeting rpsL (N20, 5′-AGAGCAGAGTTAGGCTTCTT-3′). Then the fragment was ligated upon itself to form the pgRNA6.

CRISPR/Cas9-mediated ssDNA recombineering was conducted using a two-step electrotransformation strategy. Firstly, 1 μg pgRNA5 was transformed into C. glutamicum SL4ΔldhA::rfp. The competent cells of C. glutamicum SL4ΔldhA::rfp (pgRNA5) were prepared by addition of 1 g/L sodium propionate to induce RecT recombinases expression, and then co-transformed with 1–2 μg pCas9 and 6–15 μg synthetic ssDNA (rfp-off1 or rfp-off2, Additional file 1: Table S1). Cells were recovered at 30 °C for 6 h and then spread on SGY plates supplemented with Km, Cm, and IPTG (1 mM). Plates were incubated at 30 °C for 2–3 days until colonies appeared. Recombination events were verified by detecting the fluorescence outputs of colonies. C. glutamicum SL4ΔldhA::rfp ^off1 mutants were further verified by gene sequencing. When rpsL was selected as a target of ssDNA recombineering, similar procedures described above were used with small modifications. Plasmid pgRNA6 was first transformed into C. glutamicum SL4. The competent cells of C. glutamicum SL4 (pgRNA6) was then transformed with pCas9 and synthetic ssDNA (rpsL-K43R, Additional file 1: Table S1). C. glutamicum SL4 rpsL ^K43R mutants were verified by Str^R phenotype test and gene sequencing. To perform ssDNA recombineering in C. glutamicum ATCC 13032, an engineered strain (ATCC 13032::rfp) was used and rfp was selected as a target. The procedures were similar with those for recombineering C. glutamicum SL4ΔldhA::rfp except that 0.01 mM IPTG was used for inducing Cas9 expression.

Double-locus editing

rfp and rpsL were selected as targets for double-locus editing in C. glutamicum ATCC 13032::rfp. Plasmid pgRNA7 that simultaneously expressed two gRNAs targeting rfp and rpsL was constructed by inserting a gRNA fragment targeting rpsL into pgRNA5. The gRNA fragment targeting rpsL was amplified by PCR using primer pair gRNA-8/gRNA-9 from pgRNA6. The pgRNA5 backbone was amplified by PCR using primer pair gRNA-10/pEC-XK99E-2. The two fragments were ligated to form pgRNA7. The procedures were similar with those for single-gene editing in C. glutamicum ATCC 13032 by using CRISPR/Cas9-mediated ssDNA recombineering, except that two kinds of synthetic ssDNAs (10 μg rfp-off1 and 10 μg rpsL-K43R, Additional file 1: Table S1) were transformed with pCas9 simultaneously.

Plasmid curing

To remove Cas9 and gRNA expression plasmids from edited cells, the edited colony was inoculated into 100 mL of SGY medium without antibiotics and cultivated for 12 h. The culture was serially transferred into fresh medium with an inoculum size of 0.1% (v/v) for another two times, diluted, and spread on SGY plates without antibiotics. Colonies were confirmed as cured by determining their sensitivity to Km and Cm.

ssDNA:

single-strand DNA

FACS:

fluorescence-activated cell sorting

CRISPR:

clustered regularly interspaced short palindromic repeats

Cas:

CRISPR-associated proteins

dCas9:

nuclease-deactivated Cas9

PAM:

protospacer adjacent motif

DSB:

double-strand breakage

NHEJ:

endogenous nonhomologous end joining

IPTG:

isopropyl-β-d-thiogalactopyranoside

CRISPRi:

CRISPR interference

RFP:

red fluorescent protein

SGY:

soya peptone-glucose-yeast extract

Km:

kanamycin

Cm:

chloramphenicol

SNPs:

single nucleotide polymorphisms

CDSs:

coding sequences

JL, YW, JS, and PZ conceived and designed the experiments. JL, YW, and YL performed the experiments. JL and YW analyzed the data. JS, PZ, and YM contributed reagents and analytic tools. JL, YW, JS, PZ, and YM wrote the paper. All authors read and approved the final manuscript.

Acknowledgements

We thank Dr. Meng Wang for helpful discussions.

Competing interests

The authors declare that they have no competing interests.

Availability of data and materials

All data generated or analyzed during this study are included in this published article and its additional files. The authors are willing to provide any additional data and materials related to this research that may be requested for research purposes.

Consent for publication

Not applicable.

Ethics approval and consent to participate

Not applicable.

Funding

This work was supported by the National Natural Science Foundation of China (31700044 and 31370829), the Key Research Program of the Chinese Academy of Sciences (ZDRW-ZS-2016-2), and the first Special Support Plan for Talents Development and High-level Innovation and Entrepreneurship Team of the Tianjin Municipal City.

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1. Jiao Liu and Yu Wang contributed equally to this work

Authors and Affiliations

1. Key Laboratory of Systems Microbial Biotechnology, Chinese Academy of Sciences, Tianjin, 300308, People’s Republic of China

   Jiao Liu, Yu Wang, Yujiao Lu, Ping Zheng & Jibin Sun

2. Tianjin Institute of Industrial Biotechnology, Chinese Academy of Sciences, Tianjin, 300308, People’s Republic of China

   Jiao Liu, Yu Wang, Yujiao Lu, Ping Zheng, Jibin Sun & Yanhe Ma

Corresponding authors

Correspondence to Ping Zheng or Jibin Sun.

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