Jasmonic acid and methyl jasmonate modulate growth, photosynthetic activity and expression of photosystem II subunit genes in Brassica oleracea L

The effects of jasmonic acid (JA) and methyl jasmonate (Me-JA) on photosynthetic efficiency and expression of some photosystem (PSII) related in different cultivars of Brassica oleracea L. (var. italica, capitata, and botrytis) were investigated. Plants raised from seeds subjected to a pre-sowing soaking treatment of varying concentrations of JA and Me-JA showed enhanced photosynthetic efficiency in terms of qP and chlorophyll fluorescence. Maximum quantum efficiency of PSII (Fv/Fm) was increased over that in the control seedlings. This enhancement was more pronounced in the Me-JA-treated seedlings compared to that in JA-treated ones. The expression of PSII genes was differentially regulated among the three varieties of B. oleracea. The gene PsbI up-upregulated in var. botrytis after treatment of JA and Me-JA, whereas PsbL up-regulated in capitata and botrytis after supplementation of JA. The gene PsbM showed many fold enhancements in these expressions in italica and botrytis after treatment with JA. However, the expression of the gene PsbM increased by both JA and Me-JA treatments. PsbTc(p) and PsbTc(n) were also found to be differentially expressed which revealed specificity with the variety chosen as well as JA or Me-JA treatments. The RuBP carboxylase activity remained unaffected by either JA or Me-JA supplementation in all three varieties of B. oleracea L. The data suggest that exogenous application of JA and Me-JA to seeds before germination could influence the assembly, stability, and repair of PS II in the three varieties of B. oleracea examined. Furthermore, this improvement in the PS II machinery enhanced the photosynthetic efficiency of the system and improved the photosynthetic productivity in terms of saccharides accumulation.


Results
Pre-treatment of JA and MeJA improves growth. Brassica oleracea var. capitata, botrytis, and italica seedlings treated with different levels of JA and Me-JA, responded variably in terms of root growth, shoot growth, fresh weight, dry weight, moisture content and percent biomass (Table 1). An increase of 52.69% and 43.11% in root length of B. oleracea var. capitata seedlings was observed when treated with 1 µM JA and MeJA, respectively. An increase by 58.68% and 50.29% was observed with 1 nM JA and Me-JA, respectively, as compared to the control seedlings of all cultivars. The root length increased further by 9.49% and 20.88% in response to 1 nM JA and MeJA, respectively, in comparison to that of the control seedlings. On the contrary, there was no change in root length in B. oleracea var. italica with JA supply, but root length increased to 34.61% in exposure to 1 pM MeJA as compared to that in the control seedlings (Table 1).
More specifically, in B. oleracea var. italica, the shoot length decreased by 32.07% and 18.48%, respectively, when treated with 1 µM JA or MeJA, compared to the control. When JA and MeJA were diluted to 1 nM, the inhibitory effects were minimal, and with a further dilution to 1 pM, 4.89% increase in shoot length was observed when compared to the control. On the other hand, in B. oleracea var. capitata a consistent decline in shoot length was observed for both JA and MeJA treatments. Moreover, a proportionate reduction in shoot length in the order of 2.60%, 4.55%, and 9.74%, respectively, due to treatment with 1 µM, 1 nM and 1 pM Me-JA and by 2.60%, 6.49% and 8.44%, respectively, with 1 µM, 1 nM and 1 pM JA, when compared to the control seedlings ( Table 1). The seedling biomass in terms of fresh weight and dry weight (Table 1) fluctuated depending on the concentrations of JA or MeJA in B. oleracea var. capitata. The treatment with both JA and MeJA at 1 µM improved the fresh weight by 9.58% and 10.89%, respectively, when compared with that of the control, while dry weight increased by 12.59% and 14.81% due to the treatment with 1 µM JA and MeJA, respectively, when compared to the control. Pre-treatment of JA and MeJA increased fresh weight of B. oleracea var. italica, but dry weight increased only with MeJA treatments at concentrations of 1 µM, 1 nM and 1 pM, by 19.32%, 30.68% and 63.63%, respectively, when compared to the control. Addition of 1 pM JA to B. oleracea var. italica improved its dry weight by 29.54%. Our data showed no change in dry weight of B. oleracea var. botrytis seedlings at all concentrations of JA and MeJA. A slight increase of 10.66% in dry weight was observed when treated with 1 nM MeJA. The moisture content declined in B. oleracea var. italica and capitata after pre-treatment with JA and MeJA in a dose-dependent manner. The moisture levels declined by 1.05% and 0.08% due to treatment with 1 µM JA in B. oleracea var. italica and capitata, respectively, when compared to the control. However, when B. oleracea var. botrytis seedlings were treated with 1 µM JA and MeJA, a slight increase in moisture content by 1.49% and 1.08%, respectively, was observed when compared to untreated control. In general, moisture content declined in all three cultivars when treated with JA and MeJA (Table 1). Percent biomass ( Table 1) of seedlings of all three cultivars increased. The significant decline by 20.16% and 27.26% in the seedlings raised from 1 µM treatment of MeJA and JA, respectively, was recorded in Botrytis seedlings compared with the control. B. oleracea var. italica seedlings treated with MeJA www.nature.com/scientificreports www.nature.com/scientificreports/ produced increased biomass by 11.77%, 16.81% and 29.95%, when treated with 1 µM to 1 nM and 1 pM, respectively. In B. oleracea var. italica seedlings, percent biomass was increased by 21.94% and 29.95%, when treated with 1 µM JA and 1 pM MeJA, respectively, when compared to the untreated control seedlings. B. oleracea var. capitata seedlings had no change in percent biomass with either of the treatments.

Seed priming with JA and MeJA maintains chlorophyll pigments, chl a/b, and carotenoids.
Total chlorophyll content in B. oleracea var. italica underwent a minimal change, with only a slight increase of 7.80% and 5.62% when treated with 1 pM JA and 1 nM JA, respectively, and when compared with that of the untreated control seedlings (Table 2). Reduced total chlorophyll content was observed in 1 µM JA (1.63%), and in 1 nM Me-JA (6.49%). In case of B. oleracea var. capitata, all the JA treatments (except 1 pM JA) and Me-JA increased the total chlorophyll content, with the highest increase of 5.73% observed with 1 nM JA treatment, when compared to the control seedlings (Table 2). Total chlorophyll content of B. oleracea var. botrytis increased with all JA treatments as presented in Table 2. The seedlings treated with 1 µM JA exhibited increased total chlorophyll content (1.09 ± 0.04 mg/g FW), although it was not significant in comparison to that in the control seedlings treated with distilled water (1.03 ± 0.004 mg/g FW total chlorophyll content). Treatment with Me-JA led to a general decrease in the total chlorophyll content, except 1 pM Me-JA treatment that resulted in a 9.24% increase when compared to the control seedlings. Table 2 shows that chl a/b ratio increased in seed priming with JA and MeJA treatments in B. oleracea var. botrytis and italica. In B. oleracea var. italica it increased by 5.26% and 23.22%, when primed with 1 pM JA and 1 pM Me-JA, respectively, as compared to that in the control seedlings. In B.  Table 2. Effects of Jasmonic acid (JA) and Methyl jasmonate (Me-JA) on the total chlorophyll, Chl a/b ratio, and total carotenoids of Brassica oleracea L. var.italica, capitata and botrytis. Values are means ± SD of three independent replications (n = 3). Different letters (a-e) within the column indicate statistically significant differences among the treatments, according to Tukey's test at (P < 0.05).
oleracea var. capitata similar results with JA priming were experienced. Only 1 nM JA priming led to a decrease in chl a/b ratio (5.81%), but the treatment with 1 µM and 1 pM JA increased this ratio by 3.32% and 9.11%, when compared with the control. Me-JA at all three concentrations tested led to a decrease in chl a/b ratio. In B. oleracea var. botrytis both JA and Me-JA increased the chl a/b ratio except for 1 µM JA. In the case of JA priming, 1 nM and 1pM JA increased the chl a/b ratio to almost the same level, which was 5.36% and 5.51%, respectively, as compared to that in the control seedlings. A maximum increase of 13.5% in chl a/b ratio was noted in 1 µM Me-JA supplemented seedlings as compared to the control seedlings. Carotenoid content varied depending on the treatment and concentrations of JA and MeJA used. JA at 1 nM and 1 pM increased the total carotenoid content in B. oleracea var. italica by 5.49% and 8.82%, respectively, whereas 1 µM MeJA treatment resulted in 3.09% increase compared to that in the untreated control seedlings ( Table 2). All other treatments with JA and MeJA reduced total carotenoid content when compared to the controls. In B. oleracea var. capitata, seed priming with both JA and Me JA led to an increase in total carotenoids, with the highest levels recorded for 1 nM JA (7.62%) and 1 pM MeJA (6.11%), respectively, and when compared to the control ( Table 2). The JA and MeJA treatments in B. oleracea var. botrytis showed effects contrary to that noted in B. oleracea var. italica and capitata. All the three JA treatments (1 µM, 1 nM and 1 pM) led to a reduction in carotenoid content by 5.67%, 1.58%, and 2.52%, respectively, over that in the non-primed control seedlings. In addition, 1 µM and 1 nM Me-JA treatments led to a decrease in carotenoid content by 1.21% and 2.33%, but the seedlings treated with 1 pM had increased carotenoid content by 7.79%, when compared to that in the control seedlings.
effect of JA and MeJA on chlorophyll fluorescence. Various JA and MeJA treatments had non-significant effects on the photosynthetic efficiency of PSII, appraise as Fv/Fm ratio. Brassica oleracea var. italica had the maximum increase in photosynthetic efficiency of PS II when treated with 1 nM JA (8.61%). With 1 µM MeJA treatment, Fv/Fm value increased by 8.31%, when compared to the control (Fig. 1A). In B. oleracea var. capitata, not much effect on photosynthetic efficiency of PSII was observed, the treatment with 1 nM JA and 1 pM MeJA increased the Fv/Fm ratio by 9.51% and 5.15%, respectively, when compared to the control (Fig. 1A). On the other hand, in B. oleracea var. botrytis,1 µM MeJA treatment led to 8.55% increase in Fv/Fm value. The JA priming treatment in B. oleracea var. botrytis did not alter the Fv/Fm ratio (Fig. 1A). The photosynthetic yield www.nature.com/scientificreports www.nature.com/scientificreports/ (ɸ PS II) in JA and MeJA primed treatments in all three varieties varied significantly. Brassica oleracea var. italica treated with JA had significantly reduced ɸ PS II, with the maximum reduction seen when treated with 1 nM JA (35.73%) compared with the control. However, the treatment with 1 pM JA improved ɸ PS II by 31.85% when compared to the control. The MeJA treatment at 1 µM also improved ɸ PS II by 25.72%, while 1 nM and 1 pM concentrations caused reduction in ɸ PS II by 39.04% and 36.70%, respectively, when compared to the control (Fig. 1B). In B. oleracea var. capitata, 1 µM JA priming treatment led to a 52.36% increase in ɸ PS II, while 1 µM MeJA treatment resulted only in a minor 5.57% increase over that in the control seedlings. All other JA and MeJA treatments reduced ɸ PS II in B. oleracea var. capitata compared to the control (Fig. 1B). The MeJA priming treatment was found to be generally effective in increasing ɸ PS II compared to JA in the B. oleracea var. botrytis seedlings. A notable improvement of 352.04% in ɸ PS II was observed when primed with 1 µM MeJA, compared to that of the control untreated seedlings. (Fig. 1B). Photochemical quenching was improved in the treatments with various doses of JA and MeJA in all three varieties, but the results were inconsistent. These observations show that both derivatives of JAs (JA and MeJA) increased qP in all three varieties. However, MeJA seemed to be more effective in B. oleracea var. botrytis (Fig. 1C).
Effect of JA and MeJA priming on Rubisco activity. Rubisco activity did not increase when treated with various doses of JA and MeJA in all three cultivars. In almost all the cases of exogenous JA or MeJA applications, the rubisco activity was found to be decreased. This reduction was, however, statistically non-significant ( Fig. 2A).
consequence of JA and MeJA priming on total carbohydrates, total soluble sugars, and reducing and non-reducing sugars. Seed priming with JA and MeJA led to a significant accumulation of total carbohydrates in all three cultivars of B. oleracea L. The JA and MeJA treatments at 1 µM in B. oleracea var. italic caused 47.32% and 23.70% increase in total carbohydrate content, respectively, over those in the control seedlings (Fig. 2B). In B. oleracea var. capitata, the JA and MeJA treatments led to increase in carbohydrate content by 20.37% and 34.07%, respectively, with the highest effect being at 1 nM, compared with that in the control seedlings (Fig. 2B). In B. oleracea var. botrytis, again 1 nM JA increased the total carbohydrate content by 40.45% over the control seedlings. The MeJA treatment with 1 µM led to an increase in total carbohydrates by 48.79%, compared to the control (Fig. 2B).
Total soluble sugars (TSS) increased due to the exogenous application of JA and MeJA in all three varieties. Maximum TSS accumulation was observed in B. oleracea var. italica treated with 1 µM of JA or MeJA, which was found to be increased by 34.21% or 28.82%, respectively, when compared to the control (Fig. 2C). In B. oleracea var. capitata, the treatment with 1 nM JA or MeJA resulted in the highest levels of TSS, which were 21.72% and 32.73%, respectively, when compared to the controls (Fig. 2C). In B. oleracea var. botrytis, the JA and MeJA treatments at 1 pM resulted in the highest amounts of TSS, which were 26.42% and 21.70%, respectively, compared with the control (Fig. 2C).
The content of reducing sugars (RS) increased many-folds with the JA and MeJA treatments in B. oleracea var. italica and botrytis. The JA and MeJA treatments to seeds at 1 pM led to an increase of 113.57% and 218.55% in RS, in the plants raised from the primed seeds, respectively, compared to that in the control seedlings raised from non-primed seeds (Fig. 2D). In B. oleracea var. capitata, JA and MeJA treatments had no effect on the RS content, unlike observed in B. oleracea var. italica and botrytis, but 1 pM of JA and MeJA increased RS content by 21.98% and 29.43%, respectively, compared to that of the control (Fig. 2D). The RS levels in B. oleracea var. botrytis varied significantly depending on the concentration of JA and MeJA applied. For instance, 1 pM of JA and MeJA increased RS by 349.72% and 740.88%, respectively, compared to the control (Fig. 2D).
Non-reducing sugar (NRS) content increased in B. oleracea var. italica, when treated with JA and MeJA. In the 1 µM treatment, the NRS content in the seedlings increased by 35.35% and 27.74%, respectively, compared with the control (Fig. 2E). In B. oleracea var. capitata, exogenous application of both JA and MeJA increased the NRS content., and the highest increase was observed when treated with 1 nM JA and 1 nM MeJA, with values of 22.16% and 32.67%, respectively, compared with the control (Fig. 2E). In B. oleracea var. botrytis, JA and Me-JA treatments led to an increase in NRS, albeit to a lesser extent. The maximum increase of 15.97% over control was observed in the seedlings treated with 1 nM JA. For MeJA, treatment with 1 pM resulted in the highest increase (14.13%) of NRS, and when compared to the control (Fig. 2E).

Effects of JA and MeJA priming on the expression of PsbI, PsbL, PsbM, PsbTc(p) and PsbTc(n)
genes. A few genes of PSII were examined for their expression in 10-day old seedlings of B. oleracea L. var.
italica, capitata and botrytis, raised from seeds primed with JA and MeJA. In B. oleracea L. var. italica the expression of PsbI gene was down-regulated when treated with JA or MeJA, compared to the PsbI expression in the control seedlings (Fig. 3A). In B. oleracea L. var. capitata, JA and Me-JA downregulated the PsbI expression (Fig. 4A). However, in B. oleracea L. var. botrytis, the PsbI expression was found to be upregulated in all three different treatments, which was different from that observed in B. oleracea L. var. italica and capitata. Maximum upregulation of gene expression occurred with 1 µM, followed by 1 nM, and 1 pM JA. MeJA also resulted in the upregulation of gene expression in the 1 µM and 1 nM treatments, with the maximum values obtained with 1 µM treatment. At the lowest concentration of Me-JA (1 pM), the PsbI expression was significantly down-regulated (Fig. 5A).
In B. oleracea L. var. italica, the expression of PsbL was upregulated 1.225-fold with 1 nM JA, compared to that in the control seedlings, but it was downregulated in the highest (1 µM) and lowest (1 pM) concentration of JA. At the same time, the downregulation of gene expression was noted in all MeJA priming treatments (Fig. 3B). In  (Fig. 5B).
JA treatment (1 nM) in B. oleracea L. var. italica led to upregulation in the expression of PsbM gene by 2.178-fold compared to the control seedlings. The treatment with MeJA led to downregulation of the PsbM gene expression in all priming treatments, and this increase had been in a dose-dependent manner (Fig. 3C). In B. oleracea L. var. capitata, both JA and MeJA treatments led to the upregulation of the PsbM gene expression. Maximum upregulation was observed in the seedlings resulting from the 1 µM-primed seeds, and it was upregulated by 3.031-fold compared to the control. Similar upregulation up to 4 or 5-fold was observed for the PsbM gene expression in the seedlings raised from the seeds primed with1 nM MeJA (Fig. 4C). In B. oleracea L. var. botrytis, MeJA showed a stronger effect than did JA in upregulation of the PsbM gene, and was upregulated by 1.045-fold in the seedlings raised from 1 µM MeJA-primed seeds compared with the control. The MeJA treatment at 1 pM had the highest upregulation of the PsbM gene expression, which increased by 2.428-fold compared to the control (Fig. 5C).  (Fig. 3D). In B. oleracea L. var. capitata, both JA and MeJA treatments led to the upregulation of PsbTc(p) gene expression; however, the 1 µM JA treatment had a stronger effect, and increased the expression by 3.647-fold over the control. In comparison, 1 nM of the MeJA treatment resulted only in moderate upregulation of the PsbTc(p) gene by 1.741-fold (Fig. 4D). In B. oleracea L. var. botrytis, JA priming upregulated the PsbTc(p) gene expression by 1.963-fold, and the maximum effect was observed when treated with 1 pM, compared with the control. The MeJA www.nature.com/scientificreports www.nature.com/scientificreports/ treatment with 1 nM resulted in a maximum upregulation of the PsbTc(p) gene expression by 2.796-fold over the control (Fig. 5D).
The PsbTc(n) gene expression in B. oleracea L. var. italica, was found to be upregulated with the JA and MeJA treatments. However, the MeJA treatments showed the opposite trend of upregulation. The JA treatment (1 µM) resulted in the upregulation of the PsbTc(n) gene expression by 1.941-fold, compared to the control, but the treatment with MeJA (1 pM) resulted in a maximum of this gene by 2.868-fold, compared with the control (Fig. 3E). In B. oleracea L. var. capitata, the JA treatment downregulated the expression of PsbTc(n) at all three concentrations tested. On the other hand, MeJA upregulated the PsbTc(n) gene expression by 1.366 and 1.112 folds, at 1 µM and 1 nM treatments, respectively, compared to the control (Fig. 4E). In B. oleracea L. var. botrytis, the PsbTc(n) gene expression was upregulated following the treatment with 1 µM and 1 nM, by 1.678 and 1.231-fold when compared to the control. The treatment with 1 nM of MeJA resulted in the upregulation of the PsbTc(n) gene expression by 1.392-fold, compared with the control (Fig. 5E). www.nature.com/scientificreports www.nature.com/scientificreports/

Discussion
Exogenous application of JA and MeJA had a strong influence on root length in all three cultivars of B. oleracea L.; particularly, in B. oleracea var. capitata, the root length increased by 58.68% compared to the control. Suppression of the inhibitory effect of exogenous application of JA and MeJA on primary root growth has been studied by overexpressing of NINJA and JAZ proteins responsible for the deletion, mutation, or variation in the JA domain 25 . While this might be applicable in our study, however, further validation is necessary. Unlike the root, shoot length decreased with JA and MeJA treatments, despite JA reportedly mimics auxin-like activity in regulating plant growth. The inhibitory effect of the two JA conjugates was dose-dependent, and it is being first time observed that the JAs counteraction also depends on the genetic makeup of plants, as the three cultivars of B. oleracea L. performed differently for shoot inhibition, and maximum inhibition was observed in B. oleracea var. italica. This behaviour of JA is because of the fact that it regulates shoot length by inhibiting mitotic cell division; cell elongation and cell division 26 . MeJA application to A. thaliana suspension culture repressed the activation of M phase genes and arrested the cell in G 2 phase 26,27 . Both the moisture content and the fresh weight increased due to the application of JA or MeJA. Dry weight increased mostly due to the application of JAs. Mir et al. 28 recorded similar www.nature.com/scientificreports www.nature.com/scientificreports/ results in maize plants, in which seeds affected by salinity were pre-treated with JA, after which plant growth and biomass were found to be increased.
Exogenous application of JAs enhanced photosynthetic pigments and improved the photosynthetic efficiency. However, these changes were in a dose-dependent manner. Total chlorophyll content increased the most in B oleracea L. italica, by 7.8%, particularly when treated with 1 pM JA. In B. oleracea L. capitata, it increased by 5.73% when treated with 1 nM JA. Enhanced content of chlorophyll pigments might have been due to improvement in the activities of the enzymes like proto-chlorophyllide reductase and α-aminolevulinic acid dehydratase involved in the biosynthesis of chlorophyll [29][30][31] . There are two major enzymes that regulate chlorophyll biosynthesis in higher plants, i.e. α-aminolevulinic acid dehydratase and proto-chlorophyllide reductase 31 . α-aminolevulinic acid dehydratase is a common precursor of the tetrapyrrole ring in chlorophyll structure and is known to alleviate certain stress conditions by enhancing chlorophyll synthesis 29 . On the other hand, the proto-chlorophyllide reductase is also well known to enhance the chlorophyll content of higher plants by the light-dependent protochlorophyllide reduction 30,32 . Our results contradict the findings of Cotado et al. 20 , which reported a reduction in total chlorophyll content when treated with jasmonates in Saxifraga longifolia 20 . While the effects of JA could be correlated to the accumulation of carotenoids in B oleracea L. italica and capitate. However, the carotenoid levels in B oleracea L. botrytis remained unchanged. Sirhindi et al. also observed an increase in carotenoid content due to the exogenous application of JA 33 . The relationship between photosynthesis and JA is known 32 , and the interaction of transcription factor JAZs with YABBY1 and YABBY3, which are involved in JA signalling leading to increased chlorophyll degradation 34 . JA signalling may work independent of the COI1-JAZs-MYC2/3/4 signalling cascade in B. oleracea L., however, this needs further confirmation 35 . The Chl a/b ratio increased due to exogenous priming with JA and MeJA in B. oleracea L., var. italica and botrytis, and to some extent in capitata. These findings which support the view that JA enhances the photosynthetic efficiency by increasing chlorophyll a content. Chl a is the immediate donor of photon to the reaction centres of PS II and PSI. Our results are in agreement with those of Cotado et al. 20 . Increase in chl a over chl b and to some extent the carotenoids, facilitate in maintaining the photosynthetic complex at a higher level, which further leads to an increase in sugars, particularly after treating with JA and MeJA. These results align with those of Attaran et al. 36 , who described a close relationship between the PS II quantum efficiency and expression levels of the genes involved in growth and photosynthesis 36 . No changes were observed in RuBisCO from the exogenous application of JA and MeJA in all B. oleracea cultivars. Some authors have reported a decline in RuBisCO activity due to JA or MeJA, quite similar to our findings 37 . PÉRez and Goossens 38 described the physiological role of JA-Ile by activating the JA signalling pathway in Arabidopsis. Based on varying results obtained, it is possible that different JA signalling pathways exist for JAs, and may be independent of the COI1-MYC2-JAZ co-receptor pathway 39 . Application of JA and MeJA resulted in Fv/Fm ratio of around 0.83, indicating no photoinhibition in B. oleracea L. as compared to the control. In B. oleracea L. var. italica, the photosynthetic efficiency of PS II increased due to JA and MeJA, but no changes were observed in capitata. Our results are similar to those reported in some other studies that JA promotes Fv/Fm, thereby indicating a maximal quantum efficiency of PS II 33,40,41 . Further studies are needed to investigate this in detail.
A significant increase in total carbohydrates was observed in all three cultivars of B. oleracea L. due to the application of JA or MeJA, which showed a considerable involvement of these conjugates in CO 2 fixation by these plants. Similarly, total soluble sugars also increased after treatment with JA and MeJA in all three cultivars of B. oleracea L. Accumulation of reducing sugars and to some extent non-reducing sugars by JA and MeJA reflects a regulatory role of the conjugates in photosynthetic metabolism as indicated from the observations recorded in our study. The activation level of RuBisCO in the present study after the application of JA and MeJA also supports the higher accumulation of photosynthetic products in all three cultivars of B. oleracea L., as RuBisCO is responsible for limiting photosynthetic CO 2 assimilation, and its reduced level would be responsible for wiping off the limitation in photosynthetic CO 2 assimilation. Our results are in agreement with those of Guo, et al. 42 who have reported increased RuBisCO activity that limited the photosynthetic CO 2 assimilation and photorespiration in MeJA-treated Jin1-9/myc2 plants.
A few genes involved in the regulation of PS II activity were examined after the exogenous application of JA or MeJA. We observed that PSbI was down-regulated in both italica and capitata by the JA and MeJA treatments, while it was up-regulated in botrytis. Both PsbM and PsbI are required for the efficient formation and stability of PSII dimers in vivo. They have different roles; PsbM being located in the center is required directly for the formation of dimers and its absence can lead to the instability of the dimers accumulated 13,43 . In the present study, while comparing the PS II efficiency with the expression of Psb (ɸ PSII) genes in botrytis, it was confirmed that JA and Me-JA treatment improved both function and stability of PSII, which is required for ɸ PSII enhancement. In capitata, PsbM showed up-regulation while PsbI showed down-regulation. In all the treatments of JA and Me-JA, a consistency with the photosynthetic efficiency as well as qP, i.e. photochemical quenching, being directly dependent on the formation and stability of PS II dimmer, was observed. In italica both PsbI and PsbM were down-regulated except at 1 nM JA where PsbM showed more than two-fold up-regulation. Uto et al. 43 have reported the functional role of PsbM in the stabilization of the PSII dimer and maintenance of electron transfer efficiency of PSII based on X-ray crystal structure analysis at a resolution of 4.2 Å. It was found that deletion of PsbM results in a slight widening of the lipid hole involving QB, which induces structural changes of the bicarbonate ion coordinated to the non-heme Fe(II) atom, and destabilizes the polypeptide chains around the QB binding site located far from the position of PsbM and decrease in the electron transfer rate from QA to QB in PsbM deletion mutants i.e. ∆PsbM-PSII as compared to the wild-type PSII which was interpreted on basis of structural changes caused by the deletion of the PsbM subunit. In the present study, gene expression of psbI and psbM in different concentrations of JA and Me-JA showed a direct co-regulation with PSII (ɸ PSII) efficiency as well as photochemical quenching in all three cultivars. Analysis of expression of PsbM in tobacco plants unveiled its prominent role in altering the properties of the Q B site and the electron flow within PSII rather than (2020) 10:9322 | https://doi.org/10.1038/s41598-020-65309-1 www.nature.com/scientificreports www.nature.com/scientificreports/ in the biogenesis of higher order PSII complexes in plants 12 . These differences in results suggested the presence of different signalling pathways of JAs which either involved MAPKs or Ca 2+ -calmodulin or some other protein kinases involvement might be possible in regulating gene expression responsible in PSII RC protein synthesis in different cultivars of B. oleracea. Due to this reason, dynamic regulations of the PSbI gene have been observed. Another gene PsbL, responsible for reduction reactions of PSII and Q A activity as an electron acceptor, was found to be upregulated when treated with 1 nM JA, but down-regulated with 1 µM and 1 pM concentrations of JA. In italica, PsbL expression was up-regulated at 1 nM JA concentration, while down-regulation was recorded in 1 µM and 1 pM concentrations of JA. This unveiled accountability of JA for photosynthetic machinery could also be supported by the physiological results explained above. Capitata and botrytis also showed up-regulation of PsbL, thereby strengthening the photosynthetic efficiency as well as CO 2 fixation in these two cultivars by both JA conjugates. The electron flow in PS II as well as the dimerization of the PSII reaction centre is influenced by PsbM, which was found to be up-regulated in all three cultivars. PsbTc gene, responsible for repairing PSII from photodamage, facilitating the binding of Q A with it and its reactivation after photoinhibition damages, was up-regulated when supplemented with JA or MeJA in most of the cultivars studied. PsbTc is located close to PsbM and PsbL in the dimerization domain 3 and the deletion of its gene destabilises the binding of PsbM and results in monomerization of the dimeric PSII core 44 . Ohnishi and Takahashi 45 revealed the role of this protein in the efficient post-translational repair process of photo-damaged PSII under high light conditions by comparing wild-type and a PsbTc-deficient mutant in green alga Chlamydomonas reinhardtii. More recently, its role in the early assembly steps of PSII has been shown 46 . Directed inactivation of PsbTc in tobacco plants did not prevent photoautotrophic growth, but clearly affected the PSII forward and backward electron transfer reactions, stability of PSII dimers and the assembly of PSII light-harvesting complexes (LHCII) 14 . conclusion Photosynthesis is an important metabolic process, which provides chemical energy by using sunlight for all forms of life on earth. PSII protein complex is the most important component of the photosynthetic apparatus. Its synthesis, biogenesis and management are crucial for photosynthetic efficiency, which are ultimately responsible for photosynthetic productivity in the form of different saccharides. Several reviews are available in the literature regarding the PSII assembly and repair mechanism, but as per our knowledge, no single research paper is available which discusses the assembly and stability of genes responsible for efficient formation and stability of PSII. Furthermore, no reports are available to date which would discuss the effect of plant growth regulators in maintaining the structural stability and functional efficiency of PSII in any particular crop plant. The present results suggest that Me-JA at low concentrations has more potential in making the PSII structure more stable and actively efficient as compared to JA. Besides, the genetic makeup of different varieties also matters in showing the effect of exogenous application of JA and Me-JA, which is very clear in the present study wherein three cultivars showed variable performance for the Psb gene expression as well as for photosynthetic efficiency. However, further biochemical and molecular studies are required to elucidate the adaptation of dynamic nature of PS II towards changing environmental conditions, particularly in the context of achieving enhanced crop productivity.

Material and methods
experimental set up. Viable seeds of broccoli (Brassica oleraceaL. var. italica, capitate and botrytis) were sterilized by immersing in 0.01% HgCl 2 solution for 2 min. After washing with tap water 3-4 times, the seeds were pre-soaked for 6 hrs in solution containing different concentrations (1 μM, 1 nM and 1 pM) of JA and MeJA. The seeds were arranged viz Control; 1 μM MeJA; 1 μM JA; 1 nM MeJA; 1 nM JA; 1pM Me-JA and 1pM JA. After pre-soaking the seeds were allowed to germinate in Petri plates containing Whatman's filter paper, for 3 days in a growth chamber (indosaw) with 25 °C, photoperiod of 16 h dark/light period and 80% humidity. Low light (LL) stress were initiated by providing light with the intensity of 200 μmol (photon m −2 s −1 ). The experiment was laid in randomised block design with three replicates each. The seedlings were shifted to the growth paper for 10 days after appearance of plumule. After that the seedlings were harvested for the analysis of total chlorophyll, chla/b, carotenoids, maximum quantum yield of PSII photochemistry (Fv/Fm), effective quantum yield of PSII photochemistry (ΦPSII), photochemical (qP,) non-photochemical quenching (NPQ), Rubisco activity, total carbohydrates, total soluble sugars, reducing and non-reducing sugars, and gene expression by using RT PCR.
Growth and biomass yield. Root and shoot length were measured manually using a scale. Dry weight was recorded after drying the sprouts at 70 °C for 48 h in an oven. chlorophyll and carotenoid content. Chlorophyll and carotenoids were extracted from known weight of fresh first (primary) leaf using 80% acetone. The extract was used to determine absorbance at 645, 663 and 470 nm using a spectrophotometer (Beckman 640 D, USA) 40 .
Chlorophyll fluorescence. Chlorophyll fluorescence parameters of the first (primary) leaf was determined using a portable pulse amplitude-modulated fluorimeter (Heinz Walz). The method of White and Critchley 47 was used. A dark period of 20 min was provided to the plants before measuring. Using a modulated radiation not sufficient to induce any photosynthesis in the leaf, the minimum fluorescence (F 0 ) was calculated for all PSII reaction centres (RCs) that were open. The maximal fluorescence (F m ) was measured when all RCs were closed, using a 0.8 s pulse of saturating radiation of 3000 µmol m −2 s −1 in leaves acclimatized to dark. (EC 4.1.1.39). Using the method of Usuda 48 , ribulose 1,5-bisphosphatecarboxylase/oxygenase activity was determined by monitoring NADH oxidation at 30 °C at 340 nm. Leaf tissue (1 g) was homogenized using a chilled mortar and pestle with ice-cold extraction buffer containing 0.25 M Tris-HCl (pH7.8), 0.05 M MgCl 2 , 0.0025 M EDTA, and 37.5 mg DTT. The homogenate was centrifuged at10,000×g for 10 min at 4 °C. The resulting supernatant was used for the enzyme assay. The reaction mixture (3 mL) contained 100 mM Tris-HCl (pH 8.0), 40 mM NaHCO 3 , 10 mM MgCl 2 , 0.2 mM NADH, 4 mM ATP, 5 mM DTT, 1U of glyceraldehyde 3-phosphodehydrogenase, 1 U of 3-phosphoglycerate kinase, and 0.2 mM ribulose 1,5-bisphosphate (RuBP).

Rubisco activity
Total carbohydrates, soluble sugars, reducing and non-reducing sugars. The protocol of DuBois, et al. 49 was used to estimate total carbohydrates. The OD was taken at 485 nm using a spectrophotometer (Beckman 640 D, USA). Total soluble sugars were estimated as described by Loewus 44 . The absorbance was recorded at 630 nm. The estimation of reducing sugars was done by adopting the procedure of Nelson-Somogyi 50 using a spectrophotometer (Beckman 640 D, USA) and determining absorbance at 620 nm. Non-reducing sugar content was calculated by deducting the amount of reducing sugars from the total soluble sugars and expressed as mg/g DW tissue.
Gene expression analysis. All the three varieties supplemented with JA and MeJA were further analysed by real time polymerase chain reaction (RT-PCR, Applied Biosystems). Total RNA was extracted from the leaves using GET TM Total RNA Kit. RNA concentration and purity were determined at 260 and 280 nm using the nanodrop. The first strand cDNA was prepared from 1 µg RNA template using miRNA 1 st -Strand DNA Synthesis Kit. cDNA was amplified using specific primers ( Table 3). The relative abundance of β-actin (AB047313) was also determined in order to standardise the results, which was defined as 100 relative expression units (REU) and used as the internal standard. The relative expression ratio of each gene was calculated using the comparative Ct value method 51 . The experiments were repeated twice independently, and the fold change was calculated. The relative expression value with fold change of ≥2.0 and ≤0.5 as compared to control untreated seedlings gene expression was considered to be upregulated and downregulated, respectively. Gene expression was analysed using REST. Statistical analysis. The data presented here was subjected to one-way analysis of variance (ANOVA) to analyse the effects of different concentrations of JA and MeJA. The results are expressed as the mean ± standard error of three replicates. Tukey's test (P < 0.05) was applied for the multiple comparison using Graph Pad Prism Version 7.