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Article

CRISPR/Cas9-Mediated Targeted Mutagenesis of Betaine Aldehyde Dehydrogenase 2 (BADH2) in Tobacco Affects 2-Acetyl-1-pyrroline

by
Mingli Chen
1,
Siyu Shen
2,
Zhiyuan Li
1,
Huashun Wang
2,
Jin Wang
3,
Guangyu Yang
3,
Wenwu Yang
3,
Lele Deng
3,
Daping Gong
1,* and
Jianduo Zhang
3,*
1
Tobacco Research Institute, Chinese Academy of Agricultural Sciences, Qingdao 266101, China
2
Key Laboratory of Natural Products Synthetic Biology of Ethnic Medicinal Endophytes, State Ethnic Affairs Commission, Yunnan Minzu University, Kunming 650031, China
3
Yunnan Academy of Tobacco Science, Kunming 650231, China
*
Authors to whom correspondence should be addressed.
Agronomy 2024, 14(2), 321; https://doi.org/10.3390/agronomy14020321
Submission received: 5 January 2024 / Revised: 25 January 2024 / Accepted: 27 January 2024 / Published: 1 February 2024
(This article belongs to the Special Issue Cultivation Physiology, Molecular Biology and Molecular Breeding of Solanaceae)
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Abstract

:
2-acetyl-1-pyrroline (2AP) is a highly effective volatile compound that gives fragrance to numerous plant species and food. Mutation(s) in the betaine aldehyde dehydrogenase 2 (BADH2) gene results in the accumulation of 2AP. However, the function of BADH genes in tobacco (Nicotiana tabacum L.) remains poorly understood. In this study, we successfully obtained four betaine aldehyde dehydrogenase (BADH) genes from tobacco. Phylogenetic analysis of the protein sequences showed that two of the four BADH genes were closely related to the wolfberry (Lycium barbarum) BADH gene (LbBADH1), so we named them NtBADH1a and NtBADH1b, respectively. The other two BADH genes were orthologues of the tomato (Solanum lycopersicum) aminoaldehyde dehydrogenase 2 (SlAMADH2) gene, and were named NtBADH2a and NtBADH2b, respectively. Expression analysis revealed that the biological functions of NtBADH1a and NtBADH1b were different from those of genes NtBADH2a and NtBADH2b. We introduced mutations into NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b in tobacco using the CRISPR/Cas9 system and identified transgenic Ntbadh mutant tobacco lines. Single mutants (Ntbadh1a, Ntbadh1b, Ntbadh2a and Ntbadh2b) and double mutants (Ntbadh1a-Ntbadh1b and Ntbadh2a-Ntbadh2b) harbored deletion or insertion of nucleotides, both of which led to the production of a frameshift, preventing protein accumulation. A popcorn-like scent was noticeable in tobacco leaves from the Ntbadh2a-Ntbadh2b double mutant, but not from any single mutant or the Ntbadh1a-Ntbadh1b double mutant or the wild type. Consistent with this observation, we only detected 2AP in fresh leaves from the Ntbadh2a-Ntbadh2b double mutant. These findings indicate that only the combined inactivation of NtBADH2a and NtBADH2b results in 2AP accumulation in tobacco, which was not related to NtBADH1.

1. Introduction

Betaine aldehyde dehydrogenase (BADH) is an enzyme found in a large number of plant species; it confers the potential to accumulate glycine betaine (GB), which is a powerful osmoprotectant associated with abiotic stresses, such as salt, drought, and temperature [1]. The BADH gene has been cloned from higher plants and other living organisms [2], e.g., Spinacia oleracea [3,4], Beta vulgaris [5,6], barley (Hordeum vulgaris) [7], Chenopodium quinoa [8], rice (Oryza sativa L.) [9], and Lycium ruthenicum [10]. BADH plays a crucial role in enhancing tolerance to abiotic stress by facilitating the accumulation of GB derived from betaine aldehyde (BA). In contrast, certain plant species such as tobacco (Nicotiana tabacum L.), tomato (Solanum lycopersicum L.), and rice are unable to accumulate GB owing to insufficient BA [11]. In addition to abiotic stress mechanisms, multifunctional BADH is involved in fragrance production through the polyamine oxidation pathway [12]. It has been observed that the majority of plants exhibit two BADH isozymes (BADH1 and BADH2). According to He et al., 2015 [11], there are two members of the BADH family in the rice genome: BADH1 is closely correlated with salt tolerance, while BADH2 is responsible for conferring fragrance to rice.
The 2-acetyl-1-pyrroline (2AP) is a volatile compound widespread in nature. It is the key flavor-related compound in diverse cereal products and vegetable-derived products [13,14,15]. A reduction in BADH2 activity or the presence of nonfunctional BADH2 enzymes results in the production of 2AP and the release of fragrances in rice [16], maize, sorghum (Sorghum bicolor) [17], soy-bean (Glycine max) [18], foxtail millet (Setaria italica) [19], and mung bean (Vigna radiata) [20]. The 2AP biosynthesis pathway comprises two main path-ways (Figure S1): glutamate-proline and ornithine metabolism, and polyamine metabolism. Glutamate, proline, and ornithine are converted to 1-pyrroline-5-carboxylate (P5C) via ∆1-pyrroline-5-carboxylate synthase (P5CS), proline dehydrogenase (ProDH), and ornithine aminotransferase (OAT) enzymes; P5C is then immediately converted to ∆1-pyrroline, which is the immediate precursor of 2AP and an important factor for regulating the 2AP biosynthesis rate; polyamines (organic compounds with more than two amino groups) are converted to GABald (the immediate precursor of γ-aminobutyric acid) [21]. In the presence of a nonfunctional BADH2 enzyme, GABald cannot be converted to GABA, resulting in the spontaneous conversion of GABald to ∆1-pyrroline, which leads to GABald accumulation and 2AP formation. Conversely, GABald is converted to GABA by a functional BADH2, which ultimately inhibits 2AP biosynthesis [22].
Tobacco is extensively cultivated as a non-food crop all over the world, and is additionally a crucial model plant species for fundamental biological investigation [23]. However, no genes in the 2AP biosynthetic pathway have been characterized in tobacco. Understanding the 2AP biosynthetic pathway in tobacco will help elucidate the function of 2AP in tobacco metabolism and biosynthesis. Over the past few years, genome-editing technology, such as zinc finger nucleases (ZFNs), transcription activator-like effector nucleases (TALENs), and the CRISPR/Cas9 system, which is associated with the clustered regularly interspaced short palindromic repeats (CRISPR) protein 9 (Cas9) system, has enabled scientists to make changes in the DNA of model organisms to generate biotechnologically important products [24,25,26,27]. Among these tools, CRISPR/Cas9 is widely used in plants because of its ease of use, great effectiveness, and low development cost [28]. In this study, we cloned four NtBADH genes from tobacco and characterized their roles in 2AP biosynthesis via targeted knockout using the CRISPR/Cas9 system.

2. Materials and Methods

2.1. Plant Materials

Seeds of the tobacco (Nicotiana tabacum L.) cultivar ‘Honghuadajinyuan’ and homozygous transgenic NtBADH knockout lines were surface-sterilized and grown on Murashige and Skoog (MS) Basal Medium (Duchefa Biochemie, Haarlem, The Netherlands) containing 30 g/L sucrose and 6 g/L agar. One-month-old seedlings were transferred to pots containing a peat moss to perlite ratio of 3:1 and kept under greenhouse conditions with a photoperiod of 16 h light at 25 °C. Roots, stems, leaves, and flowers of ‘Honghuadajinyuan’ seedlings were sampled at the anthesis flower stage and immediately frozen in liquid nitrogen for RNA purification.

2.2. Cloning of Tobacco NtBADH2 Genes

We acquired four NtBADH-like translated nucleotide sequences from the Sol Genomics Network (SGN) Nicotiana tabacum BX genome database (http://solgenomics.net/organism/Nicotiana_tabacum/genome, accessed on 4 January 2024) by performing a basic local alignment search tool (tBLASTn; available online: https://solgenomics.net/tools/blast/, accessed on 4 January 2024) using the rice OsBADH2 protein sequences as the query. Four full-length NtBADH coding sequences were amplified from tobacco leaf tissue cDNA by PCR using specific primers (Table S1) and 2× Phanta Max Master Mix (Vazyme, Nanjing, China). The amplified PCR products were effectively cloned into the pEASY-Blunt Zero Cloning Vector (TransGene, Beijing, China) and subjected to sequencing analysis.

2.3. Phylogenetic Analysis

Protein sequence alignments of multiple BADH orthologs from Arabidopsis thaliana, Triticum urartu, Hordeum vulgare, Oryza sativa, Zea mays, Sorghum bicolor, Cocos nucifera, Solanum lycopersicum, Solanum tuberosum, Lycium barbarum, Glycine max, Vigna radiata (Mung bean), Cucumis sativus, Cucumis melo, and Nicotiana tabacum were performed using the MUSCLE method in MEGA (version 7.0.26; https://www.megasoftware.net/, accessed on 4 January 2024) with default settings. A phylogenetic tree was reconstructed with 1000 bootstrap replicates using the neighbor-joining method of MEGA version 7.0.26.

2.4. RNA Extraction and Gene Expression Analysis

Root, stem, leaf, flower and seed tissues were collected from 60-day-old tobacco plants after transplanting to the field, immediately frozen in liquid nitrogen, and kept at 80 °C until RNA extraction. An RNAprep Pure Plant Plus Kit (Tiangen Biotech, Beijing, China) was used to isolate total RNA. A NanoDrop 2000 Spectrophotometer (Thermo Fisher Scientific, Waltham, MA, USA) was used to quantify the total RNA concentration. First-strand cDNA was synthesized using M-MLV Reverse Transcriptase (Promega, Madison, WI, USA) in a 20 μL reaction using 500 ng of starting total RNA. Quantitative reverse transcriptase PCR (qRT-PCR) was performed using SYBR Premix Ex Taq (TaKaRa Bio Inc., Otsu, Japan) and gene specific primers (Table S2) in a LightCycler® 96 instrument (Roche, Basel, Switzerland). Expression levels of the actin gene were used as an internal control. Each analysis was conducted with a minimum of three biological and technical replicates. Relative fold-change of target genes was determined by the 2−ΔΔCt method as described by Livak and Schmittgen 2001 [29].

2.5. Construction of CRISPR/Cas Gene Editing Vectors

To facilitate NtBADH genomic DNA modifications, we synthesized oligonucleotides with a specific target of two 24 base pairs in length. The CRISPOR 5.01 software (http://crispor.tefor.net/, accessed on 4 January 2024) was used to assess their efficiency. Subsequently, these oligos were annealed and inserted into the BsaI site of the enhanced pOREU3TR vector, which was optimized to enhance the expression of sgRNA cassettes and integrate a Ros1 expression cassette for efficient screening of transgene-free genome edited plants [30].

2.6. Plant Transformation and Mutant Analysis

The pOREU3TR vectors, which carried the gRNA and Cas9 expression cassettes, were introduced into Agrobacterium tumefaciens EHA105 through the freeze–thaw technique. Afterwards, positive clones were utilized in order to produce NtBADH mutant tobacco plants through the leaf discs method [31]. Seedlings resistant to kanamycin were successfully obtained and the presence of mutants was confirmed. The extracting of DNA from T0 transgenic lines was conducted using the DNeasy® Plant Mini Kit (Qiagen, Hilden, Germany). In order to detect mutations, PCR was performed using the specific primers to amplify genomic regions including the Cas9/gRNA target sites (Table S3). The products underwent sanger sequencing directly, and the resulting reads were compared with wild-type sequences to identify potential mutant lines. To investigate the heritability of CRISPR/Cas9-mediated targeted NtBADH modifications in subsequent generations, T0 lines harboring homozygous or biallelic mutations were subjected to self-pollination. Then, the T1 offspring were transferred to soil and grown until maturity for further analysis.

2.7. 2AP Measurements

2AP was quantified as in a previously described protocol [32] with slight modifications. Freeze-dried tobacco leaves were ground thoroughly into 200 mesh powder using a grinder. Aliquots (0.2 g) of ground powder were weighed into 5 mL glass bottles and extracted at 80 °C for 3 h in 2 mL of extraction buffer consisting of a 1:1 (v/v) mixture of anhydrous ethanol and dichloromethane. 2,4,6-Trimethyl pyridine (TMP) was added to the mixture at a final concentration of 50 ng/mL as an internal standard. The reaction solution was cooled to room temperature and centrifuged for 5 min at 12,000 r/min. The supernatant was transferred to an injection vial with a 200 μL internal diameter tube and left to stand for 0.5 h before measurement.
The 2AP was measured using a gas chromatograph-triple quadrupole mass spectrometer (Agilent 7890A/7000 GC-QQQ, Waldbronn, Germany) equipped with an electrospray ionization source and in separation mode using a gas chromatographic column HP-5MS (30 m × 250 μm × 0.25 μm, Agilent, Santa Clara, CA, USA). The initial column chamber temperature was set to 50 °C and held for 2 min. Then the temperature was increased to 120 °C at 10 °C min−1; finally, the temperature was increased by 30 °C min−1 to 250 °C and held for 3 min. The temperature of the injector was set to 170 °C with research grade helium (99.999%) as the carrier gas under a constant flow. The transfer line was held at 280 °C. Ions were generated using an electron impact ion source (−70 eV, 230 °C) and analyzed using a triple quadrupole. Product ion scans were acquired from 35 to 500 m/z using MRM scanning mode.

3. Results

3.1. Identification of BADH Genes in Tobacco Genome

To identify tobacco BADH gene homologues, we aligned amino acid sequences of OsBADH2 (Os08g424500) as the query against the Sol Genomics Network (SGN) tobacco genome database (http://solgenomics.net/organism/Nicotiana_tabacum/genome, accessed on 4 January 2024) using a tBLASTn search. Three putative coding sequences (mRNA_63486_cds, mRNA_31370_cds, and mRNA_66183_cds) of tobacco BADH genes were identified from the tBLASTn search. These nucleotide sequences were utilized for the purpose of designing primers that are specific to the coding sequences of BADH. These primers were then employed to amplify the full-length BADH coding sequence from tobacco leaf tissues. The tobacco BADH genes comprised four open reading frames (ORFs) that were 1515 bp, 1515 bp, 1515 bp, and 1500 bp in length and encoded proteins of 504, 504, 504, and 499 amino acids, respectively. The four BADH genes in tobacco were all predicted to consist of 15 exons and 14 introns (Figure 1).
The four tobacco BADH amino acid sequences showed high similarity at the protein level with those of other species, with NtBADH1a showing 95.24%, 92.46%, and 91.98% amino acid sequence identity with NtBADH1b, NtBADH2a, and NtBADH2b, respectively. Moreover, the tobacco BADH 1 proteins exhibited a similarity of 89.88–90.84% to LbBADH1, and the BADH 2 proteins displayed a similarity of 82.54–83.53% to LbBADH1. Meanwhile, BADH2 proteins from tobacco were 91.68–92.87% similar to SlAMADH2 and 92.28–93.47% similar to PGSC0003DMT400063025. All the encoded proteins had a highly conserved decapeptide (VTLELGGKSP) at amino acids 256–265 and a cysteine residue (C) conserved in aldehyde dehydrogenase (ALDHs) at 295 (Figure 2A).
A neighbor-joining phylogenetic tree of BADH proteins from tobacco with BADH protein from Arabidopsis thaliana, Triticum urartu, Hordeum vulgare, Oryza sativa, Zea mays, Sorghum bicolor, Cocos nucifera, Solanum lycopersicum, Solanum tuberosum, Lycium barbarum, Glycine max, Vigna radiata (Mung bean), Cucumis sativus, and Cucumis melo revealed a clear evolutionary separation between NtBADH and its homologues (Figure 2B). Two of the four BADH sequences were most closely related to LbBADH1 from Lycium barbarum and were named NtBADH1a and NtBADH1b, respectively. The other two BADH sequences had a close relationship with PGSC0003DMT400063250 from Solanum tuberosum and SlAMADH2 from Solanum lycopersicum, and were hence named NtBADH2a and NtBADH2b, respectively. Tobacco is a natural allotetraploid generated by the hybridization of Nicotiana sylvestris and Nicotiana tomentosiformis. Phylogenetic analysis showed that NtBADH1a and NtBADH2a originated from N. tomentosiformis, while NtBADH1b and NtBADH2b originated from N. sylvestris (Figure S2).

3.2. Expression Patterns of NtBADH Genes in Different Tobacco Tissues

To characterize the expression patterns of the four NtBADH genes in wild type tobacco plants, we used qRT-PCR to analyze RNA transcript levels in various tissues. We detected the four NtBADH genes transcripts in all organs. Notably, NtBADH1a and NtBADH1b had similar expression patterns, with the highest transcript levels in leaves (Figure 3A). NtBADH2a and NtBADH2b also displayed similar expression patterns and were highly expressed in seeds (Figure 3B). These results indicated that NtBADH1a and NtBADH1b might have similar biological functions in tobacco, but regulation of NtBADH1a and NtBADH1b was different from that of NtBADH2a and NtBADH2b.

3.3. Targeted NtBADH Mutations Using the CRISPR/Cas9 System

To determine the biological function of NtBADH proteins in tobacco, we decided to simultaneously knock out NtBADH1a, NtBADH1b, NtBADH2a, and NtBADH2b by genome editing with the CRISPR/Cas9 system and subsequently investigate the effect of the combinatorial mutations on the content of 2AP in tobacco. We designed three Cas9 guide RNAs, referred to as SgRNA1, SgRNA2, and SgRNA3 (20 nucleotides), and introduced these into the binary expression vector pOREU3TR. SgRNA1 and SgRNA2 independently targeted NtBADH1a and NtBADH1b, respectively. SgRNA3 had a common target site in NtBADH2a and NtBADH2b, targeting the first exon of the coding sequence for generating Ntbadh2a and Ntbadh2b single mutants and the Ntbadh2a-Ntbadh2b double mutant (Figure 4A). To generate Ntbadh1a-Ntbadh1b double mutants, we created a CRISPR/Cas9 construct harboring the SgRNA2 and SgRNA3 expression cassettes for Agrobacterium tumefaciens-mediated tobacco transformation (Figure 4B).
For NtBADH1a (sgRNA1), we identified 28 T0 positive transgenic plants through PCR amplification. Further sequencing analysis revealed that three of the plants exhibited genomic editing of the target gene with a homozygous genotype, while six plants were identified as heterozygous. Therefore, we selected the three homozygous individuals (badh1a#11, badh1a#12 and badh1a#23) for further investigation. Comparing DNA sequences revealed that badh1a#23 possessed a 22-bp deletion, badh1a#11 possessed a 1-bp deletion, and badh1a#12 exhibited 1-bp insertion at the target site, which we refer to as NtBADH1a (Figure 5A). For NtBADH1b (sgRNA2), we identified 29 T0 positive transgenic plants edited at the target site, comprising four homozygous mutants (badh1b#5, badh1b#15, badh1b#23, and badh1b#29), thirteen heterozygous mutants, and seven biallelic (two distinct variants) mutants. Individuals badh1b#5 and badh1b#15 exhibited a 1-bp insertion, and badh1b#23 and badh1b#29 possessed 1-bp and 2-bp deletions, respectively (Figure 5B).
Using the double CRISPR/Cas9 construct harboring the sgRNA2 and sgRNA3 expression cassettes, we isolated heterozygous and biallelic (two distinct variants) Ntbadh1a-Ntbadh1b double mutants at the T0 generation. To obtain edited homozygous lines, we focused on the biallelic mutations, sequencing the BADH1 target regions of 10 individual T1 transformants. We identified two types of Ntbadh1a-Ntbadh1b double mutant: a 1-bp insertion in the NtBADH1a and NtBADH1b target regions, respectively, and a 2-bp deletion in NtBADH1a and a 1-bp insertion in NtBADH1b (Figure 5C).
For NtBADH2a and NtBADH2b (sgRNA3), we screened 60 T0 transgenic lines from 63 lines using kanamycin selection. Sequencing analysis revealed 56 edited plants. Twelve edited plants showed specific editing of NtBADH2a, three of which were identified as homozygous mutant lines (badh2a#6, badh2a#17, and badh2a#18), and the remaining plants were regarded as biallelic or heterozygous mutations. Five plants showed specific editing of NtBADH2b; two of these were identified as homozygous mutant lines (badh2b#14 and badh2b#62), one possessed biallelic mutations, and the other two plants carried heterozygous mutations. Meanwhile, we identified eight homozygous plants mutated for both NtBADH2a and NtBADH2b (badh2#04, badh2#16, badh2#30, badh2#35, badh2#43, badh2#45, badh2#50, and badh2#63). The badh2a#6 line harbored a 1-bp deletion mutation, while badh2a#17 and badh2a#18 lines harbored 2-bp deletion mutations in the NtBADH2a gene only. The badh2b#14 and badh2b#62 lines carried a 1-bp deletion mutation in the NtBADH2b gene only. The double-mutant lines badh2#04 and badh2#35 contained 1-bp deletions in the NtBADH2a gene and a 2-bp deletion in the NtBADH2b gene. In the five double-mutant lines badh2#16, badh2#30, badh2#43, badh2#45, and badh2#50, the Cas9-induced mutations disrupted both the NtBADH2a and NtBADH2b genes with a 1-bp deletion mutation. The badh2#63 line contained a 1-bp insertion mutation in NtBADH2a and a 1-bp deletion mutation in NtBADH2b (Figure 5D). Importantly, all the above mutations led to frameshift mutations of NtBADH2a or NtBADH-2B.

3.4. Targeted NtBADH2a-NtBADH2b Double Mutations Affect 2AP Content

To verify the fragrance of the BADH gene-edited line, we conducted a fragrance test on fresh leaves of T0 transgenic plants with homozygous or biallelic mutations by exposing the fresh leaves to 1.7% (w/v) KOH solution for 15 min. Leaves of Ntbadh2a-Ntbadh2b double mutants had a distinctly popcorn-like fragrance compared with those of the wild type, as determined by organoleptic testing. To quantify the fragrance, we further characterized 2AP levels in leaves at the flowering stage for homozygous single or double mutants using GC-MS, with 2,4,6-trimethyl pyridine (TMP) as an internal control. As expected, we detected 2AP only in Ntbadh2a-Ntbadh2b double mutant lines, with 2AP content varying from 0.53 to 0.90 ng/mg (Figure 6A). However, levels of 2AP in any of the single mutants, the Nntbadh1a-Ntbadh1b double mutant or the wild type only varied from 0.01 to 0.05 ng/mg (Figure 6A). In addition, we further created T1 generation plants for Ntbadh2a-Ntbadh2b double mutant line badh2#16, and measured 2AP content in several tissues including the root, stem, leaf, flowers, and mature seeds. The results showed that the 2AP content in leaves was the highest with 0.71 ng/mg and was followed by the stem and flower with 0.43 ng/mg and 0.26 ng/mg 2AP content, respectively. Interestingly, the content of 2AP in seeds of double mutants was relatively low (only 0.19 ng/mg) but was still significantly higher than in the tobacco wild type. These findings indicate that only the NtBADH2 gene, and not the NtBADH1 gene, was responsible for conferring fragrance in tobacco. Furthermore, both NtBADH2a and NtBADH2b were involved in 2AP biosynthesis, and only their combined inactivation results in 2AP accumulation in tobacco.

4. Discussion

The first BADH in higher plants was isolated from Spinacia oleracea [3]. BADH contains two isoenzymes, BADH I and BADH II [33]. Previous studies have classified BADH proteins into two major branches. The members of the first subfamily are mainly from monocotyledonous plants, while the members of the other subfamily are mainly from dicotyledonous plants [34], which is consistent with our present results. We identified four BADH genes in the tobacco genome, with NtBADH1a and NtBADH1b distributed in one cluster, and NtBADH2a and NtBADH2b distributed in another cluster (Figure 2). Structural analysis of betaine aldehyde dehydrogenase in rice showed that OsBADH contains three domains: a nicotinamide adenine dinucleotide (NAD) binding domain, a substrate-binding domain, and an oligomerization domain. BADH is localized in the chloroplasts and catalyzes the oxidation of betaine aldehyde, 4-aminobutyraldehyde, and 3-aminopropanal [2]. Li et al. reported that in most plants, BADH had a highly conserved decapeptide (VTLELGGKSP) motif, which bound to cysteine (Cys) residues to determine the catalytic activity of betaine aldehyde dehydrogenase [35]. However, the decapeptides in GmBADH, ZmBADH, OsBADH, HvBADH, and SbBADH15 are VSLELGGKSP, with the second threonine residues replaced by serine [7,36,37,38,39,40]. We determined that tobacco BADH proteins contain a conserved ten-peptide motif with the sequence VTLELGGKSP, a cysteine residue (C) highly conserved in aldehyde dehydrogenases (ALDHs) that is related to enzymatic function, and an SKL motif at the C terminus, which is reported to ensure precursor protein location at peroxisomes in plants [41]. Therefore, we believe that NtBADH has similar functions to other BADH proteins and may be located within peroxisomes.
Common tobacco (N. tabacum) is an allotetraploid (2n = 48 resulting from the chromosomes sets of both parents being present in the gametes) that resulted from a Nicotiana sylvestris (2n = 24) and Nicotiana tomentosiformis (2n = 24) hybridization [42]. We determined that the tobacco genome harbors four functional BADH homologues in the present study. The phylogenetic tree revealed that two of these proteins fall within the BADH1 cluster. In contrast, the other two protein sequences were more similar to proteins in the BADH2 cluster. Although NtBADH1 and NtBADH2 were expressed in all tissues, NtBADH1 transcripts were most abundant in leaves and flowers, while NtBADH2 transcripts were most abundant in roots and seeds (Figure 3). This indicate that the function of BADH was divided in plant species. Previous studies have demonstrated that genetic mutations in BADH2 were responsible for 2AP accumulation in crops, including rice [16], soybean [43], sorghum [17] and cucumber [44]. Dysfunction of a single BADH2 copy is sufficient to confer 2AP accumulation in plant species other than maize, whose genome harbors two redundant genes, ZmBADH2a and ZmBADH2b, controlling 2AP biosynthesis [45]. In this study, we created tobacco lines by inactivating the four tobacco BADH genes by genome editing. The ntbadh2a-ntbadh2b double mutants accumulated 2AP in their leaves, flowers and kernels (Figure 6B). This is the first report to our knowledge of BADH2 genes function in tobacco. It is worth noting that NtBADH2a and NtBADH2b were highly expressed in roots and seeds, while their expression was relatively low in leaves. These expression patterns are inconsistent with previous reports in rice, sorghum and foxtail millet, where the BADH2 gene was highly expressed in leaves and panicles but showed poor expression in roots [13,19,46]. These differences suggest that the NtBADH2 gene contributes to the regulation of 2AP accumulation in a species-specific manner in tobacco.
Betaine aldehyde dehydrogenase 1 (BADH1), a homologous gene to BADH2, has been found to play a role in salt stress by facilitating the accumulation of biosynthesized glycine betaine (GB), which is known to participate in the response to abiotic stresses [47,48]. However, there are divergent findings from various studies in rice regarding the correlation between BADH1 and salt stress tolerance. Studies by Bradbury et al., 2008 showed that rice BADH1 has very low activity on BA, but the function and mechanism of BADH1 action were uncertain [49]. Meanwhile, Singh et al., 2010 argued that BADH1 is associated with rice fragrance [9]. The function of BADH1, therefore, needs further study. BADH1 in tobacco was not associated with 2AP accumulation because the content of 2AP did not change in either single Ntbadh1a or Ntbadh1b lines or double Ntbadh1a-Ntbadh1b mutant plants (Figure 6A). Whether BADH1 is a candidate gene associated with abiotic stresses in tobacco, such as salt, drought, and temperature, will be the focus of our research in the future.
The accumulation of 2AP can also be affected by growth conditions, which can regulate the expression of genes or the enzymes activity involved in 2AP biosynthesis. Conditions of alternating wetting and moderate drying [50] or low light treatment [51] significantly increase 2AP concentration. Additionally, 2AP contents of aromatic rice grains were increased under foliar application of zinc via promotion of the activity of P5CS, proline de-hydrogenase, and diamine oxidase enzymes [52]. Molybdenum can also enhance 2AP contents in rice grains through the promotion of nitrogen utilization and assimilation, stimulation of glutamate synthase activity, and elevation of proline content [53]. Conversely, drought stress [51] and cadmium stress [53] cause various inhibitory effects in rice, such as reducing 2AP contents. In addition, Maize lines carrying similar presumed loss-of-function alleles, was lower in the XCW175 inbred line than in Zheng58 and LN005M, suggesting that even genotypes carrying loss-of-function or weak alleles of the BADH2 gene may still accumulate different levels of 2AP [45]. Likewise, the same badh2 mutant could potentially accumulate varying levels of 2AP under diverse circumstances. The same may hold true in tobacco. As illustrated in Figure 6, changes in 2AP content observed in Ntbadh2a-Ntbadh2b double mutants over different generations may reflect different growth conditions. Even more importantly, 2AP content in tobacco leaves was significantly higher than in other tissues (Figure 6B); tobacco (Nicotiana tabacum) demonstrates adaptability, effective manipulation of genetic material, regeneration ability, and the capability to generate substantial quantities of leaf biomass. These characteristics contribute to achieving high levels of desired proteins, thereby simplifying the process of protein extraction and purification. Consequently, tobacco is regarded as an excellent candidate for plant-based protein production [54]. In the future, tobacco leaves may be utilized as a bioreactor under optimal conditions to enhance the accumulation of 2AP by editing additional genes involved in the 2AP biosynthetic pathway.

5. Conclusions

In summary, we successfully identified four NtBADH genes (NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b) from tobacco cultivar ‘Honghuadajinyuan’. To the best of our knowledge, this study is the first to report 2AP contents in tobacco. Our results demonstrate that NtBADH2 genes, but not NtBADH1 genes, are required for 2AP accumulation in tobacco, while NtBADH2a and NtBADH2b are redundant genes controlling 2AP biosynthesis in tobacco. In addition, we generated tobacco lines with stable and high 2AP content using CRISPR-Cas9-mediated gene knockout. The mutants in this study could be used for advanced engineering to produce unusual 2AP phenotypes.

Supplementary Materials

The following supporting information can be downloaded at: https://www.mdpi.com/article/10.3390/agronomy14020321/s1. Figure S1: The hypothetical mechanism of the synthesis of 2AP by BADH. Figure S2: Phylogenetic tree of NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b amino acid sequences with BADH proteins from N. tomentosiformis and N. sylvestris. Table S1: Specific primers used for amplifying the four full-length NtBADH gene in tobacco. Table S2: Gene-specific primers used for analysis of expression levels of four NtBADH genes. Table S3: Specific primers for mutant analysis of CRISPR/Cas9-mediated mutant lines.

Author Contributions

Conceptualization, M.C., S.S., H.W., D.G. and J.Z.; methodology, M.C., J.Z., Z.L. and J.W.; software, S.S., Z.L. and G.Y.; validation, D.G., J.Z. and W.Y.; formal analysis, S.S. and L.D.; investigation, Z.L., J.W., G.Y. and W.Y.; data curation, M.C., S.S. and L.D.; writing—original draft preparation, M.C.; writing—review and editing, J.Z., D.G., S.S. and H.W.; visualization, Z.L.; supervision, D.G. and J.Z.; project administration, M.C., D.G. and J.Z.; funding acquisition, M.C., D.G. and J.Z. All authors have read and agreed to the published version of the manuscript.

Funding

This research was funded by Special Funds for Basic Scientific Research of the Central Public Welfare Research Institutes, grant No. 1610232023013.

Data Availability Statement

Data are contained within the article or Supplementary Materials.

Conflicts of Interest

The authors declare no conflicts of interest.

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Figure 1. Putative exon/intron structure of NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b genes.
Figure 1. Putative exon/intron structure of NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b genes.
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Figure 2. Characterization of NtBADH2 protein in tobacco (Nicotiana tabacum). (A) Alignment of the putative NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b amino acid sequences with LbBADH1, SlAMADH2 and PGSC0003DMT400063250 sequences. (B) Phylogenetic tree of NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b amino acid sequences with known BADH proteins from other plant species. Nt, Nicotiana tabacum; At, Arabidopsis thaliana; Tu, Triticum urartu; Hv, Hordeum vulgare; Os, Oryza sativa; Zm, Zea mays; Sb, Sorghum bicolor; Cn, Cocos nucifera; Sl, Solanum lycopersicum; St, Solanum tuberosum; Lb, Lycium barbarum; Gm, Glycine max; Cs, Cucumis sativus. The colored lines represent motifs and the red boxes represent the conserved decapaptide (VTLELGGKSP) and a cysteine residue (C).
Figure 2. Characterization of NtBADH2 protein in tobacco (Nicotiana tabacum). (A) Alignment of the putative NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b amino acid sequences with LbBADH1, SlAMADH2 and PGSC0003DMT400063250 sequences. (B) Phylogenetic tree of NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b amino acid sequences with known BADH proteins from other plant species. Nt, Nicotiana tabacum; At, Arabidopsis thaliana; Tu, Triticum urartu; Hv, Hordeum vulgare; Os, Oryza sativa; Zm, Zea mays; Sb, Sorghum bicolor; Cn, Cocos nucifera; Sl, Solanum lycopersicum; St, Solanum tuberosum; Lb, Lycium barbarum; Gm, Glycine max; Cs, Cucumis sativus. The colored lines represent motifs and the red boxes represent the conserved decapaptide (VTLELGGKSP) and a cysteine residue (C).
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Figure 3. NtBADH expression patterns in different tissues. (A) Relative gene expression of NtBADH1a and NtBADH1b in different tissues of ‘Honghuadajinyuan’ tobacco plants. (B) Relative gene expression of NtBADH2a and NtBADH2b in different tissues of tobacco plants. R, root; ST, stem; L, leaf; F, flower; S, seed.
Figure 3. NtBADH expression patterns in different tissues. (A) Relative gene expression of NtBADH1a and NtBADH1b in different tissues of ‘Honghuadajinyuan’ tobacco plants. (B) Relative gene expression of NtBADH2a and NtBADH2b in different tissues of tobacco plants. R, root; ST, stem; L, leaf; F, flower; S, seed.
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Figure 4. CRISPR/Cas9-mediated NtBADH knockout in tobacco. (A) NtBADH gene structure and target site selected for targeted NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b mutations. Black rectangles represent exons, black lines show introns, black arrow indicate target sites, and nucleotides in red are followed by the PAM (proto-spacer adjacent motif). (B) CRISPR/Cas9 vector structure.
Figure 4. CRISPR/Cas9-mediated NtBADH knockout in tobacco. (A) NtBADH gene structure and target site selected for targeted NtBADH1a, NtBADH1b, NtBADH2a and NtBADH2b mutations. Black rectangles represent exons, black lines show introns, black arrow indicate target sites, and nucleotides in red are followed by the PAM (proto-spacer adjacent motif). (B) CRISPR/Cas9 vector structure.
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Figure 5. Sequences of the wild type and gene-edited mutants of NtBADH in the ‘Honghuadajinyuan’ background. (A) Ntbadh1a single mutants. (B) Ntbadh1b single mutants. (C) Ntbadh1a-Ntbadh1b double mutants. (D) Sequences of NtBADH2a and NtBADH2b in Ntbadh2a and Ntbadh2b single mutants and Ntbadh2a-Ntbadh2b double mutants. Guide RNA sequences are indicated in green; PAM sequences are indicated in red; italics indicates an insertion mutation; and a short transverse line indicates a deletion mutation.
Figure 5. Sequences of the wild type and gene-edited mutants of NtBADH in the ‘Honghuadajinyuan’ background. (A) Ntbadh1a single mutants. (B) Ntbadh1b single mutants. (C) Ntbadh1a-Ntbadh1b double mutants. (D) Sequences of NtBADH2a and NtBADH2b in Ntbadh2a and Ntbadh2b single mutants and Ntbadh2a-Ntbadh2b double mutants. Guide RNA sequences are indicated in green; PAM sequences are indicated in red; italics indicates an insertion mutation; and a short transverse line indicates a deletion mutation.
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Figure 6. (A) Relative contents of 2AP in the leaves of the single or double mutants and the wild type ‘Honghuadajinyuan’. (B) The 2AP content in different tissues at the flowering stage for the double mutant Ntbadh2a-Ntbadh2b line badh2#16. R, roots; ST, stems; YL, young leaves; F, flowers; S, seeds.
Figure 6. (A) Relative contents of 2AP in the leaves of the single or double mutants and the wild type ‘Honghuadajinyuan’. (B) The 2AP content in different tissues at the flowering stage for the double mutant Ntbadh2a-Ntbadh2b line badh2#16. R, roots; ST, stems; YL, young leaves; F, flowers; S, seeds.
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Chen, M.; Shen, S.; Li, Z.; Wang, H.; Wang, J.; Yang, G.; Yang, W.; Deng, L.; Gong, D.; Zhang, J. CRISPR/Cas9-Mediated Targeted Mutagenesis of Betaine Aldehyde Dehydrogenase 2 (BADH2) in Tobacco Affects 2-Acetyl-1-pyrroline. Agronomy 2024, 14, 321. https://doi.org/10.3390/agronomy14020321

AMA Style

Chen M, Shen S, Li Z, Wang H, Wang J, Yang G, Yang W, Deng L, Gong D, Zhang J. CRISPR/Cas9-Mediated Targeted Mutagenesis of Betaine Aldehyde Dehydrogenase 2 (BADH2) in Tobacco Affects 2-Acetyl-1-pyrroline. Agronomy. 2024; 14(2):321. https://doi.org/10.3390/agronomy14020321

Chicago/Turabian Style

Chen, Mingli, Siyu Shen, Zhiyuan Li, Huashun Wang, Jin Wang, Guangyu Yang, Wenwu Yang, Lele Deng, Daping Gong, and Jianduo Zhang. 2024. "CRISPR/Cas9-Mediated Targeted Mutagenesis of Betaine Aldehyde Dehydrogenase 2 (BADH2) in Tobacco Affects 2-Acetyl-1-pyrroline" Agronomy 14, no. 2: 321. https://doi.org/10.3390/agronomy14020321

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