Genes with Cold Shock Domain from Eutrema salsugineum (Pall.) for Generating a Cold Stress Tolerance in Winter Rape (Brassica napus L.) Plants "2279

The increased demand in vegetable oil for food purposes and high-protein feed for livestock and poultry encourages producers to expand the production of various oil crops, while occupying rather cold agroclimatic zones. Improved cold and frost resistance of cultivated crops would significantly increase the yield and expand the range of rape cultivation in a number of cold climate regions. Nine transgenic lines of winter rape containing genes encoding proteins with a cold shock domain (CspA иEsCSDP3) were obtained as a result of Agrobacterium transformation. In total, 260 explants were involved in transformation of rape using pBI121-CSPA-plant, with a transformation efficiency of 2.3%; among 750 explants using the pBI-EsCSDP3 construction, the efficiency was 0.4%. As a result of the studies, it was shown that the expression of the new gene Escsdp3 from the plant of Eutrema salsugineum was able to increase the cold and frost resistance of plants as effectively as the cspa gene from E. coli, which is classically used for this purpose. The cold resistance analysis of T1 transgenic plants generation revealed four cold resistant winter rape lines (three lines with the cspA-plant gene and one line with the Escsdp3 gene). The transfer of Escsdp3 and cspA-plant genes into winter rape plants led to a significant increase in frost resistance of plants. Two winter rapeseed lines were resistant to freezing (with the cspA-plant gene and with the Escsdp3 gene). Non-hardened transgenic plants remained viable after 24 h of exposure to negative temperatures up to −5 ◦C, and plants that passed through the hardening stage survived after freezing at −16 ◦C.


Introduction
Most of the total land on Earth (about 64%) has an average minimum temperature <0 • C [1]. The need for a constant increase in food production while reducing natural resources necessitates the production of plants that can withstand adverse conditions, including the effects of low temperatures.
Such abiotic stress as cold stress, including chilling (0-15 • C) and freezing (<0 • C), negatively affects the growth and agricultural productivity of plants and limits their geographical distribution [2]. Frost tolerance is understood as the ability of plants to tolerate adverse winter conditions without damage [3,4]. Cold stress usually restricts plant growth and development. Frost tolerance of plants is determined by their ability to survive during short-term frosts or prolonged frosts and depends on hereditary characteristics. which is associated with their RNA-chaperone activity [27], including the ability to melt the secondary structures of RNA and DNA [26,29,32]. In a study of the ability of EsCSDP1-4 proteins to specifically interact with nucleic acids, the unique ability of the cold shock domain of EsCSDP3 protein was found to effectively restore the growth of mutant strain E. coli (BX04 strain) cells at low temperatures. Thus, in the studies of Taranov et al. [39], of the six studied cold shock domains of A. thaliana and E. salsugineum proteins, only one, EsCSD3, showed activity in the complementation test for E. coli cell growth of the BX04 strain, similar to that of the native bacterial protein CspA. Freezing is a strongly stress-damaging, including to the contents of the cell nucleus. DNA structures containing alternating one and two strand sequences of nucleic acids are quite often formed as a result of destabilization of the DNA double helix, which require reparations. In an article by Zlobin et al. [40], it was shown that among the EsCSDP1-4 studied, only EsCSDP3 protein demonstrated high melting activity of partially double-stranded DNA. In all likelihood, the ability to nuclear localization of EsCSDP3 and its DNA-melting activity indicate a possible participation in the mechanisms associated with the reparation of the destabilized DNA structures [40].
We assumed that the protein EsCSDP3 was able to have a significant role in the formation of resistance to cold stress. The purpose of our work was to assess the potential effectiveness of using EsCSDP3 to add additional cold and frost resistance to agricultural crops. As a plant-reference with increased cold resistance, it was decided to use transgenic rape plants expressing an efficiently increased cold resistance bacterial protein CspA. The potential for resistance to cold stress in transgenic rape was evaluated in the heterozygous T 1 generation. Winter rape was chosen as the object under study, as a crop in the life cycle of which cold stresses are critical and, at the same time, a necessary part of the vegetation season. As a result, heterozygous transgenic T 1 rapeseed lines with EsCSDP3 expression were obtained, which were not inferior in cold and frost resistance to T 1 rapeseed lines with CspA expression.

Gene Synthesis and Plasmid Construction
The vector constructs pBI121-CSPA-plant ( Figure 1a) and pBI-EsCSDP3 ( Figure 1b) were created on the basis of pBI121 vector by replacing the ß-glucoronidase synthesis gene which also has the target cspA gene isolated from Escherichia coli with the optimized codon composition for the plants of the cabbage family (Brassicaceae) (cspA-plant) and the target Escsdp3 gene, encoding the protein with the cold shock domain of E. salsugineum [40,41], respectively.
Agronomy 2021, 11, x FOR PEER REVIEW 3 of 20 "short" proteins (EsCSDP2 and EsCSDP4) with two ZnFs [39], the functional activity of which is associated with their RNA-chaperone activity [27], including the ability to melt the secondary structures of RNA and DNA [26,29,32]. In a study of the ability of EsCSDP1-4 proteins to specifically interact with nucleic acids, the unique ability of the cold shock domain of EsCSDP3 protein was found to effectively restore the growth of mutant strain E. coli (BX04 strain) cells at low temperatures. Thus, in the studies of Taranov et al. [39], of the six studied cold shock domains of A. thaliana and E. salsugineum proteins, only one, EsCSD3, showed activity in the complementation test for E. coli cell growth of the BX04 strain, similar to that of the native bacterial protein CspA. Freezing is a strongly stress-damaging, including to the contents of the cell nucleus. DNA structures containing alternating one and two strand sequences of nucleic acids are quite often formed as a result of destabilization of the DNA double helix, which require reparations.
In an article by Zlobin et al. [40], it was shown that among the EsCSDP1-4 studied, only EsCSDP3 protein demonstrated high melting activity of partially double-stranded DNA. In all likelihood, the ability to nuclear localization of EsCSDP3 and its DNA-melting activity indicate a possible participation in the mechanisms associated with the reparation of the destabilized DNA structures [40]. We assumed that the protein EsCSDP3 was able to have a significant role in the formation of resistance to cold stress. The purpose of our work was to assess the potential effectiveness of using EsCSDP3 to add additional cold and frost resistance to agricultural crops. As a plant-reference with increased cold resistance, it was decided to use transgenic rape plants expressing an efficiently increased cold resistance bacterial protein CspA. The potential for resistance to cold stress in transgenic rape was evaluated in the heterozygous T1 generation. Winter rape was chosen as the object under study, as a crop in the life cycle of which cold stresses are critical and, at the same time, a necessary part of the vegetation season. As a result, heterozygous transgenic T1 rapeseed lines with EsCSDP3 expression were obtained, which were not inferior in cold and frost resistance to T1 rapeseed lines with CspA expression.

Gene Synthesis and Plasmid Construction
The vector constructs pBI121-CSPA-plant ( Figure 1a) and pBI-EsCSDP3 ( Figure 1b) were created on the basis of pBI121 vector by replacing the ß-glucoronidase synthesis gene which also has the target cspA gene isolated from Escherichia coli with the optimized codon composition for the plants of the cabbage family (Brassicaceae) (cspA-plant) and the target Escsdp3 gene, encoding the protein with the cold shock domain of E. salsugineum [40,41], respectively.

Optimization of the Codon Usage of the cspA Gene
The amino acid sequence of the protein, which is 77 amino acids, was taken from the GenBank (GenBank: AIF96121.1). The encoding CspA protein nucleotide sequence, which is optimal for plants of Brassicaceae (Figure 2), was established using the JCat program [42]. Further on we amplified the full-length cspA-plant gene sequence, flanked by the VspI restriction site at the 5 -end and the BamHI at the 3 -end, by "PCR-based accurate synthesis (PAS) of long DNA sequences" [43]. for the synthesis of neomycin phosphotransferase (nptII) is under the control of the regulatory elements of the nopaline synthase gene (NOS-pro).

Optimization of the Codon Usage of the cspA Gene
The amino acid sequence of the protein, which is 77 amino acids, was taken from the GenBank (GenBank: AIF96121.1). The encoding CspA protein nucleotide sequence, which is optimal for plants of Brassicaceae (Figure 2), was established using the JCat program [42]. Further on we amplified the full-length cspA-plant gene sequence, flanked by the VspI restriction site at the 5′-end and the BamHI at the 3′-end, by "PCR-based accurate synthesis (PAS) of long DNA sequences" [43].

Mutant Bacteria Growth Complementation
The synthesized cspA gene was cloned into the pINIII expression plasmid vector [25] using the VspI restriction sites at the 5′-end and BamHI at the 3′-end, by standard procedures. The resulting genetic construct was designated as pINIII-cspA(plant). The genetic construct based on the pINIII vector containing the native cspA gene (pINIII-cspA) was described previously [39]. Cells of the quadruple mutant E. coli BX04 (ΔcspA, ΔcspB, ΔcspE, ΔcspG) were transformed by pINIII-cspA(plant), pINIII-cspA constructs, and original pINIII vector to test the codon-optimized cspA-plant gene and to restore growth ability at low temperature (+ 17 °C). The transformed cells were grown in a liquid medium (LB) in the presence of the antibiotics ampicillin (0.2 g L −1 ) and kanamycin (0.05 g L −1 ) up to an optical density of OD550 = 0.8, then the multiplied cells were diluted to the concentrations of 10 −1 , 10 −2 , 10 −3 , 10 −4 , 10 −5 , and 10 −6 , and after that, the cell amount of 7 μL was applied onto the surface of solid LB medium in Petri dishes containing ampicillin (0.2 g L −1 ), Km (0.05 g L −1 ), and isopropyl β-D-1-thiogalactopyranoside (0.2 M). The plates were incubated at 17 °C for five days.

Creation of Genetic Constructs for Overexpression
The genetic construct harboring the cspA-plant gene was amplified with the DNA of the pINIII-cspA(plant) plasmid using the primers 5′-ATTGGATCCACCCTTTTT-GGCTGTTTCCTCTC-3′ with the BamH1 restriction site (underlined) and 5′-TAA-GAGCTCTTAAGCAAGCGAAGAACATTCCCT-3′ with the Sac1 restriction site (underlined). The obtained PCR fragment was cloned into the pBl121 vector at the restriction

Mutant Bacteria Growth Complementation
The synthesized cspA gene was cloned into the pINIII expression plasmid vector [25] using the VspI restriction sites at the 5 -end and BamHI at the 3 -end, by standard procedures. The resulting genetic construct was designated as pINIII-cspA (plant) . The genetic construct based on the pINIII vector containing the native cspA gene (pINIII-cspA) was described previously [39]. Cells of the quadruple mutant E. coli BX04 (∆cspA, ∆cspB, ∆cspE, ∆cspG) were transformed by pINIII-cspA (plant) , pINIII-cspA constructs, and original pINIII vector to test the codon-optimized cspA-plant gene and to restore growth ability at low temperature (+ 17 • C). The transformed cells were grown in a liquid medium (LB) in the presence of the antibiotics ampicillin (0.2 g L −1 ) and kanamycin (0.05 g L −1 ) up to an optical density of OD 550 = 0.8, then the multiplied cells were diluted to the concentrations of 10 −1 , 10 −2 , 10 −3 , 10 −4 , 10 −5 , and 10 −6 , and after that, the cell amount of 7 µL was applied onto the surface of solid LB medium in Petri dishes containing ampicillin (0.2 g L −1 ), Km (0.05 g L −1 ), and isopropyl β-D-1-thiogalactopyranoside (0.2 M). The plates were incubated at 17 • C for five days.

Creation of Genetic Constructs for Overexpression
The genetic construct harboring the cspA-plant gene was amplified with the DNA of the pINIII-cspA (plant) plasmid using the primers 5 -ATTGGATCCACCCTTTTTGGCTGTTTCCTCTC-3 with the BamH1 restriction site (underlined) and 5 -TAAGAGCTCTTAAGCAAGCGAAGAACATTCCCT-3 with the Sac1 restriction site (underlined). The obtained PCR fragment was cloned into the pBl121 vector at the restriction sites BamH1 and Sac1; the nucleotide sequence of the resulting genetic construct was verified by sequencing.
Isolation of total RNA, cDNA synthesis, and PCR amplification of Escsdp3 was performed to create a genetic construct that included the coding part of the Escsdp3 gene. Total RNA was isolated from the leaves of the Eutrema salsugineum using Trizole reagent (Invitrogen, Carlsbad, CA, USA) in accordance with the manufacturer's protocol. cDNA was obtained by reverse transcription using SuperScript III revertase (Invitrogen, Carlsbad, CA, USA). Amplification of the Escsdp3 gene was performed using primers 5 -ATTGGATCCACCCTTTTTGGCTGTTTCCTCTC-3 with the BamH1 restriction site (underlined) and 5 -TAAGAGCTCTTAAGCAAGCGAAGAACATTCCCT-3 with the Sac1 restriction site (underlined). The resulting PCR fragment was cloned into a pGEM-T vector. Its nucleotide sequence was checked by sequencing, and then recloned into the pBl121 vector for agrobacterial transformation at the BamH1 and Sac1 restriction sites.

Tissue Culture, Agrobacterium-Mediated Transformation, and Obtaining Generation T 0
The research was carried out using Russian winter rape of the "Severyanin" variety ( ® 9811769, domestic selection created at FWRC FPA). It is the first double-zero ("00") variety to be used in the Central region of Russia.
Sterile seedlings of rape were used to produce plant explants. Seeds were sterilized superficially for 35 min by 30% water solution of sodium hypochlorite, then 5-fold washed with sterile water and subsequently placed on agarized basal Murashige and Skoog medium (MS) [45] for germination and growth in vitro. Hypocotyls with a size of 7 mm were excised from 15-day-old seedlings and placed for precultivation on agarized MS medium supplemented with 1.0 mg·L −1 2,4-D (2,4-dichlorophenoxyacetic acid) [46] for further Agrobacterium-mediated transformation.
Experiments were conducted by co-cultivation of explants (precultured hypocotyls) jointly with Agrobacterium tumefaciens suspension. An overnight culture of A. tumefaciens was prepared in 50 mL of liquid YEB medium, supplemented with 100 mg·L −1 Km and 50 mg·L −1 rifampicin, and shaken in an orbital shaker (180 rpm) within 24 h at 28 • C in the dark. Then it was diluted with sterile distilled water to a final concentration at an optical density of OD 600 = 0.4-0.6. The explants were placed into a flask containing 50 mL of inoculum and kept for 30 min in an orbital shaker (100 rpm) for inoculation. After drying in air flow laminar box, the explants were transferred onto filter paper, placed on a solid surface of MS medium supplemented with 1.0 mg·L −1 2,4-D in Petri dishes, and co-cultivated in light conditions at a temperature of 21 • C for 72 h. After co-cultivation period, the explants were washed with liquid MS medium, with a lack organic components but supplemented with 300 mg·L −1 Tm, and then transferred to the medium for explants cultivation and elimination of Agrobacterium (MS medium containing 1.0 mg·L −1 2,4-D and 150 mg·L −1 tmimentine (Tm) with the addition of 100 mg·L −1 kanamycin sulfate (Km)). Two weeks later, the explants were transferred to regeneration medium-MS medium supplemented with 4.0 mg·L −1 N 6 -benzyladenine, mg·L −1 Zeatin, 5.0 mg·L −1 AgNO 3 [47], and 150 mg·L −1 Tm and 100 mg·L −1 Km. Every 2 weeks, explants were transferred to fresh media.
The resulting Km-resistant regenerants were rooted in a half-strength MS medium with a lack of organic components and supplemented with 0.5 mg·L −1 indole-3-butyric acid and 100 mg·L −1 Km.

Adaptation, Growing Plants In Vivo, and Obtaining Generation T 1
In vitro plants were adapted to in vivo conditions. For this purpose, rooted plants were planted in a greenhouse in pots filled with soil (normalized peat + 10% agroperlite) and cultivated at 100% humidity under a protective plastic cone. After 5-7 days, the cone was removed, and plants were grown to obtain seed generation T 1 . After adaptation, the plants were transplanted into large growing containers filled with soil and grown in a greenhouse until they reached the phenological phase of readiness for owerwintering (formation of the fifth-sixth layer of leaves). Then the plants were transferred to the cold compartment of the greenhouse (+8 • C) to undergo the owerwintering stage for 2 months, after which the plants were returned to the compartment of the greenhouse, where the temperature was maintained at +25 • C for flowering. As the peduncles formed, insulators were put on the plants to avoid over-pollination and to obtain full-fledged T 1 generation seeds. For detecting the sequences of cold shock proteins (cspA-plant and Escsdp3) gene and checking T 1 plants for possible hybrid origin (to exclude the possibility of both cold shock proteins genes' presence in a single genome), PCR was performed with the simultaneous use of four sets of primers (CSDP-F, CSDP-R, CSPA-F, and CSPA-R); the reaction conditions are described above. The products were separated in 1.2% agarose gel using the electrophoresis systems.

Semiquantitative RT-PCR (Reverse Transcriptase PCR) and Quantitative RT-PCR Analyzes of Transgenic Rapeseed (Real-Time qPCR)
The selection of plant material for analysis was performed twice (before and after hardening of plants), as noted in Figure 3 (point 1 and 2). RNA samples were extracted from leaves of transgenic and control T 1 generation plants using GeneJET Plant RNA Purification Mini Kit (Thermo Fisher Scientific, Waltham, MA, United States). Each sample was treated with DNAse (Thermo). The cDNA was synthesized using Revert Aid Minus Reverse Transcriptase (Thermo) according to the manufacturer's protocol using oligo(dT) 18 and Random (dN) 10 primers. For each sample, 3 µg of total RNA was taken for the reverse transcription reaction in a total volume of 20 µL following 2-fold dilution. An amount of 2 µL of three nucleic acid preparations (cDNA mix for the study of gene expression, mRNA mix and total DNA for control of reaction) was used for PCR reaction. House-keeping Actin-7 (LOC106418315, NCBI Reference Sequence: XM_013858992.2) gene was used as internal control. RT-PCR was performed using primer sets for cold shock proteins (cspA-plant and Escsdp3) genes as described below. The respective primers sequences for Actin-7 were Act7(BNRT)F: 5 -GATTGAGCATGGTATTGTAAGC-3 and Act7(BNRT)R: 5 -CATCTTCTCCCTGTTAGCCTTA-3 (anticipated amplification fragment of 154 bp); those for Escsdp3 were DP3(BNRT)2F: 5 -CATTACTCCCGATGACGGC-3 and DP3(BNRT)2R: 5 -TCGCTTCCCAGAGTGATTGC-3 (anticipated amplification fragment of 154 bp); those for cspA-plant were PA(BNRT)F: 5 -ATGTCTGGAAAGATGACTGG-3 and PA(BNRT)R: 5 -CCTTAGATCCATCATCAGGAG-3 (anticipated amplification fragment of 157 bp). Real-Time qPCR was performed using primer sets for cspA-plant (PA(BNRT)F and PA(BNRT)R), Escsdp3 (DP3(BNRT)2F and DP3(BNRT)2R) and Actin-7 (Act7(BNRT)F and Act7(BNRT)R) gene as described above. PCR cycles were chosen so that none of analyzed samples reached a plateau at the end of the amplification; that is, they were in the ex- ponential phase of amplification. The experiments were performed on a LightCycler 96 instrument (Roche Diagnostics GmbH, Mannheim, Germany) using the qPCRmix-HS SYBR containing HS Taq polymerase and intercalating dye SYBR Green I (Evrogen, Moscow, Russia) in a volume of 20 µL. The PCR reaction conditions and the melting analysis of the products were selected according to the manufacturer's recommendations. The 2 −∆∆CT method [49] was used to normalize and calibrate the cold shock proteins (cspA-plant and tscsdp3) gene values relative to the endogenous control. Every sample was analyzed in triplicate. Data calculation and statistical analysis were performed using both the software supplied with the Roche device (LightCycler ® 96 Software 1.1 copyright F. Hoffmann-La Roche AG, Basel, Schweiz) and Microsoft Excel 2007 (copyright Microsoft Corporation, Redmond, Washington, DC, USA).

Southern Blot Analysis
T 1 generation rape genomic DNA (50 µg) was isolated from 1 g of rapeseed plant leaves cultivated in protected ground. Isolation was carried out using a buffer containing CTAB detergent according to the procedure described in Plant Molecular Biology Manual [50]. DNA concentration was measured using a spectrophotometer Thermo Evolution 260 BIO (Waltham, MA, USA). An amount of 40 µg of DNA of the selected lines and control plants were hydrolyzed overnight at 37 • C by the EcoRI enzyme (100 units) in a volume of 500 µg.
In the transferred T-DNA, the site of the selected restriction occurs once. The hydrolysis products were separated overnight by electrophoresis in 0.9% agarose gel at a voltage of 18V in the chamber Amersham MINNIE GEL UNIT (Amersham, UK). After that, the DNA was transferred to a positively charged Amersham Hybond N + membrane (GE Healthcare, UK) by capillary method, as described in the instructions for the membrane. DNA was fixed on the membrane by incubation for 2 h at 80 • C. Probes for hybridization were prepared from PCR products using the AlkPhos Direct Labeling Kit (GE Healthcare, Amersham, UK). PCR products (186 bp and 512 bp) that were amplified using primers for PCR analysis were used to detect the cspA and Escsdp3 genes. The integration of the nptII kanamycin resistance gene was confirmed using a probe consisting of 381 base pairs, which was generated using PCR and primers (5 -GCTATGACTGGGCACAACAGACAATC-3 and 5 -TCCGAGTACGTGCTCGCTCGA-3 ). Pre-hybridization and hybridization were performed at a temperature from 56 • C to 64 • C, depending on the probe. DNA-probe hybridization was performed overnight. The membrane was washed in accordance with the instructions for the set (AlkPhos Direct Labeling Kit). The membrane was placed in a reagent CDP-Star (GE Healthcare, UK). For signal accumulation, the membrane in CDP-Star solution was placed overnight in a photographic cuvette with a Retina XBE blue sensitive X-ray film (Carestream Health, Rochester, New York, NY, USA) at room temperature. The X-ray film was scanned using an EPSON Perfection V750 PRO scanner (Suwa, Nagano, Japan).

Study of Plant Resistance to Cold and Frost Plant Selection
After germination of T 1 generation seeds in the presence of 650 mg·L −1 Km, 60 resistant plants of each line were selected for assays to determine the expression level of heterologous genes and to identify the effectiveness of introduced genes for increasing the cold and frost resistance of transgenic rapeseed lines. The seeds of the control plants were germinated in Petri dishes on filter paper moistened with distilled water.
Plants were frozen in a climatic chamber Celsius 10.0 (6 adult plants for each experimental line and control-non-transgenic plants of winter rape varieties "Severyanin"). Testing temperatures were achieved by reducing the initial cultivation temperature by 2 • C h −1 (Figure 3b,c) (from +17 • C (point 1 in Figure 3a) or +4 • C (point 2 in Figure 3a) for different batches of plants). Then the plants were kept at negative temperatures for 24 h, (−3, −4, −5 • C for unhardened plants (Figure 3b) and −8, −12, −16 • C for hardened plants (Figure 3c)). After that, the temperature in the chamber was increased up to +4 • C at a rate of 2 • C h −1 (Figure 3b,c). Leaf die cuts were taken from a newly formed leaf (the second leaf from the growth point along the central vascular bundle) for potentiometric analysis of the electrolytes outflow and detection of plant tissues damage by means of light microscopy. After that, the plants were kept at +4 • C for a further 24 h and then transferred to the greenhouse (16/8 h photoperiod, 21/21 • C temperature). A week later the total moisture content of plants was assessed.

Potentiometric Analysis of Electrolyte Leakage from Plant Tissue
Potentiometric analysis of electrolyte leakage from plant tissue was carried out using the method of Dexter et al. [51]. Selected die cuts were washed with distilled water and placed into falcon tubes (10 mL) with the addition of 5 mL of distilled water. The open tubes were then placed into a Bunsen flask and, by means of an IKA MVP10 basic pump, a vacuum of 15 mbar was created in the flask for 30 min, until the air bubbles completely left the solution and die-cuts, and the die-cuts dropped to the bottom of the tube, which led to the outflow of electrolytes through the damaged cell wall into distilled water. After that, the electrical conductivity of water in test tubes with cutouts (g1) was measured using the Ohaus Starter 300C device (Parsippany, NJ, USA). Next, the sample tubes were closed and autoclaved and then the conductivity of water in the tubes was re-measured, thereby determining the total electrolyte content in the sample (g2). The loss of cell electrolytes was calculated by the formula A = g1 g2 × 100% [52].

Light Microscopy and Tissue Preparation
The inspection of the selected plant material for detection of cold damage was carried out by light microscopy. The leaf fragments containing a central vascular bundle were fixed in 2.5% (w/v) glutaraldehyde dissolved in 0.1M phosphate buffer (pH 7.2), supplemented with 1.5% (w/v) sucrose. Then plant material was washed and postfixed in 1% (w/v) OsO 4 , dehydrated in ethanol with increasing concentrations (30, 50, 70, 96, 100%), and subsequently in propylene oxide. Explants were stained with 0.1% methylene blue water solution and embedded in a mix of the epoxide resin Epon-812 and Araldite for light microscopy. Samples were studied and photographed with the use of an Olympus BX51 microscope (Olympus, Shinjuku, Tokyo, Japan) equipped with Color Viev II camera (Soft Imaging System, Munster, Germany).

Analysis of Moisture Retention in Plants
The dry matter and, accordingly, moisture content were assessed by the standard method (drying to a constant weight at 80 • C). The moisture content rate (1 unit) was taken as such in plants unexposed to cold stress (c2). The entire above-ground part of the tested plants subjected to cold stresses (including dead leaves) was dried a week after freezing (c1) to analyze the moisture content. The moisture content of the samples was determined by the formula W = c1 c2 × 100%.

Synthetic Gene and Plasmid Construction
The cspA gene sequence was optimized for expression in cabbage plants and was used to construct the pBI121-CSPA-plant construct. The functional activity of the synthesized gene was verified using the test for the restoration of growth ability in the fourth mutant E. coli (BX04: ∆cspA, ∆cspB, ∆cspE, ∆cspG) at low temperature (17 • C). Figure 4 shows that changes in the codon composition of the cspA gene did not affect the ability of the CspA protein to restore the growth of mutant bacteria of strain BX04 at low temperature. A positive test result indicates that the synthesized cspA-plant gene encodes a functionally active protein.
plants subjected to cold stresses (including dead leaves) was dried a week after freez (c1) to analyze the moisture content. The moisture content of the samples was determi by the formula W= c1 c2 100%.

Synthetic Gene and Plasmid Construction
The cspA gene sequence was optimized for expression in cabbage plants and w used to construct the pBI121-CSPA-plant construct. The functional activity of the syn sized gene was verified using the test for the restoration of growth ability in the fou mutant E. coli (BX04: ΔcspA, ΔcspB, ΔcspE, ΔcspG) at low temperature (17 °C). Figu shows that changes in the codon composition of the cspA gene did not affect the abilit the CspA protein to restore the growth of mutant bacteria of strain BX04 at low temp ture. A positive test result indicates that the synthesized cspA-plant gene encodes a fu tionally active protein.

Agrobacterium-Mediated Transformation
As a result of the studies, nine kanamycin-resistant lines were obtained. PCR analysis revealed six transgenic rapeseed lines with the introduction of the T-DNA from pBI121-CSPA-plant (A19/3, A23/2, A17-1/2, A17-1/1, A17-2, and A10-5) construction and three lines with the insertion of the plasmid pBI-EsCSDP3 T-region (D6-1/1.2, D6/1, and D-H2). In total, 260 explants were involved in transformation of rapeseed using pBI121-CSPA-plant, and transformation efficiency was 2.3%, which is common for significant crop cultivars [53]. Seven hundred and fifty explants were involved in the transformation of rapeseed with the pBI-EsCSDP3 construction, and the efficiency was 0.4%. Apparently, already at the stage of transient synthesis, the protein CSDP3 negatively affects the regeneration potential of explants.
The obtained rapeseed lines were adapted to in vivo conditions and planted into a greenhouse to obtain seed of T 1 generation for further analysis on determination of the heterologous genes expression level and to reveal the efficiency of introduced genes on increasing of the cold resistance in transgenic rapeseed lines.

Analysis of Transformants
All transgenic lines of T 1 generation were analyzed by PCR analysis and Southern blot. The fragments of the expected size were amplified from the DNA of all analyzed transgenic lines. As it was shown by PCR, all of the nine lines contained only one type of the target cold shock gene sequence ( Figure 5), which proves their non-hybrid status, despite flowering without significant spatial isolation in the greenhouse. transgenic lines. As it was shown by PCR, all of the nine lines contain the target cold shock gene sequence ( Figure 5), which proves their non spite flowering without significant spatial isolation in the greenhouse.
Integration of the cspA-plant, Escsdp3, and nptII genes into the gen rapeseed plants wsa confirmed by Southern blotting (Figure 6). The cs gration is shown in six lines (Figure 6a). The copy number of the gen lines. Thus, in lines A17-1/2, A17-1/1, and A10-5 there is a single cop gene, and in line A19/3 there are six copies, in line A23/2 there are five A17/2 there are four copies of the gene.  Integration of the cspA-plant, Escsdp3, and nptII genes into the genome of Severyanin rapeseed plants wsa confirmed by Southern blotting (Figure 6). The cspA-plant gene integration is shown in six lines (Figure 6a). The copy number of the gene varies among the lines. Thus, in lines A17-1/2, A17-1/1, and A10-5 there is a single copy of the cspA-plant gene, and in line A19/3 there are six copies, in line A23/2 there are five copies, and in line A17/2 there are four copies of the gene.
During the hybridization with a probe specific to the Escsdp3 Arabidopsis gene, a plurality of bands appeared on the membrane both in the control and in the selected lines (D6/1, D6-1/1.2, and D-H2), which significantly complicated the detection of the target signals on the membrane (Figure 6c, additional signals marked as red tick). Most likely it is due to the high homology of the transgene from Arabidopsis with the native genes of cold shock rapeseed proteins, as well as to the great diversity of these genes in the plant genome. An additional probe specific to the nptII gene was further used to more accurately confirm the transgenic status of the plants. It was found that there was a single copy insertion in line D6/1, two copies in line D6-1/1.2, and seven copies in line D-H2 (Figure 6b). However, the nptII gene was not detected in the DNA of untransformed rapeseed. Based on the profile of the bands obtained by hybridization, all lines are the result of an independent transformational event. During the hybridization with a probe specific to the Escsdp3 Arabidopsis gene, a plurality of bands appeared on the membrane both in the control and in the selected lines (D6/1, D6-1/1.2, and D-H2), which significantly complicated the detection of the target signals on the membrane (Figure 6c, additional signals marked as red tick). Most likely it is due to the high homology of the transgene from Arabidopsis with the native genes of cold shock rapeseed proteins, as well as to the great diversity of these genes in the plant genome. An additional probe specific to the nptII gene was further used to more accurately confirm the transgenic status of the plants. It was found that there was a single copy insertion in line D6/1, two copies in line D6-1/1.2, and seven copies in line D-H2 ( Figure  6b). However, the nptII gene was not detected in the DNA of untransformed rapeseed. Based on the profile of the bands obtained by hybridization, all lines are the result of an independent transformational event.
Expression of target genes was shown in all transgenic lines by means of RT-PCR (Figure 7a,b). Actin-7 was used as a reference gene. The signal of its expression on the cDNA matrix indicates the reactivity of the samples prepared for analysis. The absence of a signal on the original mRNA matrix confirms the purity of the cDNA samples that were used and indicates the reliability of the data obtained (Figure 7c). The equal size signals on the electrophoregram from the amplification products on the DNA and cDNA matrix of Escsdp3 (Figure 7a) and cspA-plant (Figure 7b) genes indicates the correctness of PCR and reliably confirms the presence of target gene expression in all obtained transgenic lines. Expression of target genes was shown in all transgenic lines by means of RT-PCR (Figure 7a,b). Actin-7 was used as a reference gene. The signal of its expression on the cDNA matrix indicates the reactivity of the samples prepared for analysis. The absence of a signal on the original mRNA matrix confirms the purity of the cDNA samples that were used and indicates the reliability of the data obtained (Figure 7c). The equal size signals on the electrophoregram from the amplification products on the DNA and cDNA matrix of Escsdp3 ( Figure 7a) and cspA-plant (Figure 7b) genes indicates the correctness of PCR and reliably confirms the presence of target gene expression in all obtained transgenic lines.
The method of quantitative evaluation of the expression of Escsdp3 and cspA-plant genes largely confirmed the results obtained with semi-quantitative RT-PCR. Expression of target genes was detected in all transgenic lines. The highest content mRNA of Escsdp3 and cspA-plant genes in all lines was detected in non-hardened samples. Two lines (A19/3 and D6-1/1.2) showed a significantly higher level of target genes expression relative to the other lines (in hardened and non-hardened samples). The expression of Escsdp3 in D6-1/1.2 line was an order of magnitude higher than in the transgenic lines D6/1 and D-H2 (Figure 8).

Study of Plant Resistance to Cold and Frost
Our studies have shown that low temperatures up to −4 • C do not adversely affect unhardened winter rape plants of the Severyanin variety. The critical temperature at which plant death begins is −5 • C (Figure 9a and Table 1). Cold damage to the leaf becomes critical and leads to rupture of the mesophyll tissue (Figure 9f, highlighted by blue arrows), and in the stomatal apertures it leads to peeling of the membrane and cell contents from the cell wall, and consequently to complete cell necrotization (Figure 9k, highlighted by blue arrows).

Study of Plant Resistance to Cold and Frost
Our studies have shown that low temperatures up to −4 °C do not adversely affect unhardened winter rape plants of the Severyanin variety. The critical temperature at which plant death begins is −5 °C (Figure 9a and Table 1). Cold damage to the leaf becomes critical and leads to rupture of the mesophyll tissue (Figure 9f, highlighted by blue arrows), and in the stomatal apertures it leads to peeling of the membrane and cell contents from the cell wall, and consequently to complete cell necrotization (Figure 9k, highlighted by blue arrows). As a result, the loss of electrolytes in leaf tissues of non-transgenic plants and a number of transgenic lines (A17-1/2, A17-1/1, A17/2, D6/1, and D-H2) exceeds the critical level of 46% (Table 1); thus, the plant loses its ability to retain moisture in the tissues. After a week, such plants are unable to retain even 60% of the initially moisture content (Table 1), which leads to wilting and drying of plant green mass (Figure 9a). After cold freezing at −5 °C, only four lines of transgenic rapeseed plants (А19/3, A23/2, A10-5, and D6-1/1.2) remained alive (Figure 9b-e). In these lines, mesophyll tissue ruptures were local and insignificant (in Figure 9g-j, they are highlighted by red arrows). In the region of the stomatal apertures, membrane peeling was observed only in a small number of cells adjacent to the aperture (in Figure 9m-n, it is indicated by orange arrows) or had a partial character (in Figure 9l-o, it is indicated by green arrows).   Non-transgenic rape plant that was not subjected to freezing was used as a reference; its values were taken as 100%. Fatal results are marked in red.
As a result, the loss of electrolytes in leaf tissues of non-transgenic plants and a number of transgenic lines (A17-1/2, A17-1/1, A17/2, D6/1, and D-H2) exceeds the critical level of 46% (Table 1); thus, the plant loses its ability to retain moisture in the tissues. After a week, such plants are unable to retain even 60% of the initially moisture content (Table 1), which leads to wilting and drying of plant green mass (Figure 9a). After cold freezing at −5 • C, only four lines of transgenic rapeseed plants (A19/3, A23/2, A10-5, and D6-1/1.2) remained alive (Figure 9b-e). In these lines, mesophyll tissue ruptures were local and insignificant (in Figure 9g-j, they are highlighted by red arrows). In the region of the stomatal apertures, membrane peeling was observed only in a small number of cells adjacent to the aperture (in Figure 9m-n, it is indicated by orange arrows) or had a partial character (in Figure 9l-o, it is indicated by green arrows).
Hardening has led to a significant increase in frost resistance of plants. Thus, after freezing at −8 • C, all lines except the A17/2 line remained alive ( Table 2); after cold processing at −12 • C, lines A19/3, A 10-5, D6-1/1.2, and D6/1 survived (lines A17-1/2, A17-1/1, A17/2, A23/2, D-H2 and the wild-type control plant died). Only two transgenic lines (A19/3 and D6-1/1.2) remained alive after freezing at a temperature of −16 • C. After freezing at this temperature, those lines showed the lowest outflow of electrolytes (the loss did not exceed 28.2% for the line D6-1/1.2 and did not exceed 34.7% for the line A19/3 ( Table 2). A week after stress, the proportion of retained moisture in tissues was 66.7% in line D6-1/1.2 and 63.5% in line a 19/3 ( Table 2). Damages at the cellular level were similar in nature to those presented in Figure 8 for plants of those lines and wild type. Non-transgenic hardened rape plant that was not subjected to freezing was used as a reference; its values were taken as 100%. Fatal results are marked in red.

Discussion
Cold is an environmental factor that limits the geographical distribution and growing season of many plant species, and it often adversely affects crop quality and productivity [54]. Genes involved in protection or repair mechanisms could be new targets for the improvement of plant plasticity and adaptive responses to stress [55]. Finding new genes responsible for abiotic stress tolerance phenotypes is of great importance not only for a better understanding of stress responses but also for promising future crop improvement [17]. Transgenic technologies have opened up many interesting possibilities for increasing resistance to cold stress in plants by introducing or removing a gene or genes that control a particular trait [56]. They also provide unique opportunities to improve the genetic potential of plants by creating specific crop varieties that are more resistant to cold stress. Over the past two decades, a number of genes have been identified that can increase plant resistance to cold [34][35][36][37].
In this work, we investigated the previously found Escsdp3 gene [38][39][40] from the extremophyte plant E. salsugineum for the effectiveness of its application for imparting additional cold resistance and frost resistance to agricultural crops. Data on the level of mRNA content of the Escsdp3 gene in plant tissues correlate with data on cold and frost resistance of the corresponding transgenic lines. Thus, the line with the highest expression of the Escsdp3 gene (D6-1/1.2) demonstrated the highest cold and frost resistance among all tested lines with introduction of the T-DNA from pBI-TsCSDP3 (D6/1 and D-H2) construction into the rape genome. The transfer of Escsdp3 gene into winter rape plants led to a significant increase in frost resistance of hardened plants and had a weak effect on unhardened plants. One transgenic line (D6-1/1.2) with expression of the Escsdp3 gene remained alive after freezing 24 h at −16 • C, while the wild type completely died after freezing 24 h at −12 • C.
Kim et al. [57] obtained a similar result when overexpressing the AtCSDP3 gene in Arabidopsis. However, according to their data, overexpression of AtCSDP3 increased the survival of both hardened and non-hardened Arabidopsis plants equally by 1-2 • C. The difference with our results is most likely not due to the differences in the amino acid sequences of the EsCSDP3 and AtCSDP3 proteins (91% identity) but to the differences in methods for measuring frost resistance and plant growth. In the aforementioned work, the resistance was assessed on ten-day-old seedlings grown under aseptic conditions on an artificial medium with the addition of 2% sucrose, while our experiments were carried out on six-week-old plants grown in soil and at the phenophase of readiness for hardening and owerwintering.
Our results indicate the prospects of using these genes and the possibly of using the other CSD protein genes in crop biotechnology in order to increase their resistance to low-temperature stress. Our studies show how the scope for further improving the traits of traditional plants cultivars can be widened using cold shock domain proteins. For further research aimed at improving the cold resistance of plants, we are going to obtain and study transgenic plants with integration into genome DREB1 and Escsdp3 genes under the control of the stress-inducible rd29A promoter [58,59]. We assume that the use of plant inducible regulatory elements will have a positive effect on improving cold resistance in transgenic crops.