WO2013114407A2

WO2013114407A2 - Primer for amplifying enone oxidoreductase from mango

Info

Publication number: WO2013114407A2
Application number: PCT/IN2013/000072
Authority: WO
Inventors: Vidya Shrikant GUPTA; Ram Shridhar KULKARNI; Ashok Prabhakar GIRI; Keshav H PUJARI
Original assignee: Council Of Scientific & Industrial Research
Priority date: 2012-02-03
Filing date: 2013-02-01
Publication date: 2013-08-08
Also published as: EP2809809A2; IN2012DE00304A; WO2013114407A3; US20160002685A1; US9790526B2; EP2809809B1

Abstract

The present invention disclosed herein the primers for amplifying enone oxidoreductase, having sequence selected from the group consisting of Seq. ID No. 1 to 13, from mango. Also disclosed herein is a novel nucleotide sequence of Sequence ID No. 14 encoding said amplified enone oxidoreductase, for enzyme production in an artificial system thus generating the desired flavor in food products.

Description

PRIMER FOR AMPLIFYING ENONE OXIDOREDUCTASE FROM

MANGO

FIELD OF THE INVENTION

The present invention relates to primer sequence for amplifying enone oxidoreductase derived from mango and an isolated nucleotide sequence encoding said Enone Oxidoreductase (EO) derived from Mangifera indica.

BACKGROUND OF THE INVENTION

Flavor is one of the most important attributes that decides the acceptability of various food items that we consume. The sensation of flavor perceived is generally because of the mixture of many chemicals in the food. Still, there are some compounds, which dominate the flavor of a particular food item and thus are themselves capable of eliciting a similar response in humans to that induced by food material. Furanones, which are found in many food products, represent one such dominating class of flavor compounds. Furanones are also important as naturally occurring flavor compounds. They are responsible for the caramel-like flavor of many fruits including strawberry, pineapple, raspberry, grapes, tomato, kiwi and mango. In addition to having a sweet and pleasant odour, furanones, especially furaneol and mesifuran, are characterized by a low odour detection threshold.

Earlier studies demonstrated that ripe mango fruits also contain high amounts of furaneol (4-hydroxy-2,5-dimethyl-3(2H)-furanone) and its methyl ether, mesifuran (2,5-dimethyl-4-methoxy-3(2H)-furanone). The fruits of cultivar Alphonso contained higher amounts of these compounds than any other cultivar and ripening of Alphonso fruits was characterized by de novo appearance and increase in the levels of these two furanones. Although furanones are not quantitatively the most dominant compounds of Alphonso fruits, the low odour detection threshold of furanones makes their contribution to Alphonso mango flavor, in terms of odour units, about 20-fold greater than that of any other volatile compound.

In spite of such crucial involvement of furanones in determining the flavor of mango and the other fruits, the biosynthesis of furaneol and mesifuran has until now been studied only in strawberry and tomato. Earlier studies on strawberry showed that out of several radiolabeled substrates fed to the ripening strawberry fruits, fructose- 1 ,6- diphosphate had the highest rate of incorporation into furaneol. This, along with the other studies confirmed fructose- 1,6-diphosphate as a natural precursor of furanones in the plants.

Further studies carried out to understand the biosynthesis of furaneol in plants indicate that fructose- 1 ,6-diphosphate is first converted by an unknown enzyme into an unstable intermediate 4-hydroxy-5-methyl-2-methylene-3(2H)-furanone (HMMF). The furaneol forming enzyme, enone oxidoreductase which is highly similar to the NAD(P)H:quinineoxidoreductase, then reduces the exocyclic α, β unsaturated bond of HMMF, resulting in the formation of furaneol. Enone oxidoreductases from both, strawberry and tomato are capable of converting various derivatives of HMMF, substituted at the methylene group, into their respective saturated products. The presence of HMMF has also been detected in the fruits such as pineapple and raspberry suggesting that the biosynthetic pathway of furanones might be similar in different plants.

Furaneol further contributes to the fruit flavor by being converted into its methyl ether, mesifuran. The enzyme responsible for the formation of mesifuran is known only from strawberry and it was shown to be an S-adenosyl methionine dependent methyl transferase that methylates the hydroxy 1 group of furaneol.

An article titled "Functional characterization of enone oxidoreductases from strawberry and tomato fruit" by Klein D., published in J. Agric Food Chem. 2007 Aug 8; 55(16): 6705-1 1 reports that HMMF, the substrate of FaEO that is formed during strawberry fruit ripening, was also detected in tomato and pineapple fruit by HPLC-ESI-MSn.

An article titled "Characterization of NAD(P)H-dependent Enone oxidoreductase of strawberry and tomato fruit" by Klein D., characterizes Fragaria ananassa enone oxidoreductase (FaEO) as an enzyme able to carry out two different reaction mechanisms depending on the available substrate. The enzyme from strawberry and a similar enzyme from tomato were heterologously expressed in E. coli, purified and biochemically characterized. The heterologously expressed enzyme catalyzed the formation of HDMF from D-fructose- 1 ,6-biphosphate and NADH.

An article titled "Alternative oxidase from mango (Mangifera indica, L.) is differentially regulated during fruit ripening" by Cruz-Hernandez A and Gomez-Lim MA published in Planta. 1995; 197(4):569-76, discloses analysis of alternative oxidase at the molecular level during the ripening of mango. Synthetic oligonucleotides, corresponding to conserved regions of the Sauromatum guttatum and Arabidopsis thaliana nucleotide sequences, were used as primers for polymerase chain reaction to amplify genomic DNA extracted from mango leaves. The 623-bp fragment was found to encode an open reading frame of 207 amino acids. Using this fragment one full-length cDNA clone, designated pAOMI. l , was obtained. The predicted amino-acid sequence exhibited 62, 64 and 68% identity to the S. guttatum, soybean, and A. thaliana enzymes respectively, indicating that this cDNA encodes a mango homologue of the alternative oxidase.

An article titled, "Ethylene biosynthesis and respiration during ripening in mango cultivars" by Reddy et. al. published in Indian Journal of Plant Physiology, 2001 , Volume 6(4), 361-364, discloses the determination of enzymatic activities of ACC- oxidase and ACC-synthase at different stages of ripening in two varieties of mango fruits {Mangifera indica L.), viz. Amrapali and Dashehari. Among the two cultivars - Dashehari showed higher level of ACC-synthase and ACC accumulation, and low level of ACC-oxidase, and ethylene production compared to Amrapali during the ripening process.

An article titled, "Expression profiling of various genes during the fruit development and ripening of mango' by Pandit et.al. published in Plant Physiology and Biochemistry, 48 (2010) explores several flavor related genes along with a few associated to the physiology of developing and ripening in 'Alphonso' mango. The temporal and spatial regulation of the genes during development and ripening of 'Alphonso' mango has been analyzed. As seen from the above disclosures, nucleotide sequence encoding enone oxidoreductases (EO) which play an important role in the biosynthesis of furaneol in mango is not known hitherto and there is a long standing need in the prior art for such sequences. Hence the Inventors have attempted in this research to provide artificial sequences which may be used to impart color, flavor and smell as in natural Alphonso mangoes.

SUMMARY OF THE INVENTION

The main object of the present invention is to provide a primer sequ ence for amplifying enone oxidoreductase derived from mango.

Another object of the present invention is to provide a nucleotide sequence encoding enone oxidoreductase enzyme having an important role in the biosynthesis of furaneol in mango, for enzyme production in artificial system, for semi-biosynthesis of flavors.

Yet another object of the present invention is to provide a novel nucleotide sequence encoding enone oxidoreductase (EO) from mango, which is useful for enzyme production in an artificial system, for semi-biosynthesis of flavors, as well as and for improving various varieties of mango.

Accordingly, the present invention provides a primer sequence for amplifying enone oxidoreductase derived from mango selected from the sequence of Seq. ID No. 1 -13. In another aspect, the present invention provides the nucleotide sequence, Seq ID No. 14, encoding enone oxidoreductase enzyme having an important role in the biosynthesis of furaneol in mango for enzyme production in artificial system, for semi-biosynthesis of flavors.

In yet another embodiment of the present invention, use the sequences for semi- biosynthesis of flavors.

In still another embodiment of the present invention, use the sequences for enzyme production in artificial system.

In yet another embodiment of the present invention, use the sequences for improving mango varieties. It is therefore an object of another aspect, to provide a novel nucleotide sequence encoding enone oxidoreductase (EO) from mango which is useful for enzyme production in an artificial system, for semi-biosynthesis of flavors, as well as for improving various varieties of mango.

Accordingly, in an aspect, the invention provides a novel nucleotide sequence encoding enone oxidoreductase derived from mango.

In another aspect, the present invention provides forward and reverse degenerate primers for enone oxidoreductase for the amplification of the cDNA prepared from ripe fruits of mango.

In yet another aspect, the present invention provides forward and reverse gene specific primers for enone oxidoreductase for the amplification of the ends of cDNA by rapid amplification of cDNA ends (RACE).

Yet another aspect, the current invention provides primers corresponding to the terminal regions of the mRNA which are designed for enone oxidoreductase. These terminal primers are used for the PCR amplification with mango cDNA as a template.

In yet another aspect, the invention provides a process of isolating gene sequence encoding functional enone oxidoreductase from mango.

In a further aspect, the invention provides process of biochemical characterization of the enone oxidoreductase isolated from mango.

BRIEF DESCRIPTION OF THE DRAWINGS

Figure 1: Complete open reading frame encoding enone oxidoreductase isolated from mango.

Figure 2: Alignment of the in silico translated sequence of /ΈΟ with the closest characterized sequences from other plants.

Figure 3: GC-MS analysis of the products formed by EO. Depicted are traces (m/z 128) of samples of authentic furaneol (a), the products of reaction catalyzed by the protein expressed from MiEO (b) and the products of reaction catalyzed by protein extract from E. coli with the plasmid carrying the reverse-oriented insert (c) In a separate analysis, total ion spectra were obtained. The spectra represented are of the authentic furaneol (d) and of the furaneol detected in the assay with MiEO (e). The presence of m/z 70, 83 and 98 in (e) was because of the contaminating co- eluent; these ions were also detected at the same time in (c).

Figure 4: Mesifuran content and relative abundance of MiEO transcripts in the ripening fruits of Alphonso mango from the three cultivation localities, Dapoli, Deogad and Vengurle in India (DAH: days after harvest. Letters indicate the significance of ANOVA (p<0.01) for the comparison between the ripening stages for the levels of mesifuran (x, y, etc.) and the relative transcript abundance of MiEO (a, b, etc.); the values having different letters are significantly different from each other.

DETAILED DESCRIPTION OF THE INVENTION

The invention will now be described in detail in connection with certain preferred and optional embodiments, so that various aspects thereof may be more fully understood and appreciated.

In order to provide a clear and consistent understanding of the specification, the following definitions are provided. Unless otherwise defined herein, all technical and scientific terms used here have the same meaning as commonly understood by one skilled in the art to which the invention belongs.

'Enone oxidoreductase' refers to an enzyme that catalyzes reduction of an enone compound.

MiEO i n the specification refers to enyme Enone oxidoreductase derived from Mangifera indica

In an embodiment, the present invention discloses a novel nucleotide sequence encoding enone oxidoreductase isolated from mango. The nucleotide sequence encoding enone oxidoreductase is useful for enzyme production in an artificial system, plays an important role in the biosynthesis of furaneol in mango. Further, the artificially synthesized enzyme can be mixed appropriately with the food product, thus generating the desired flavor. The nucleotide sequence is also useful in the flavor industry for semi-biosynthesis of flavors via various approaches such as enzyme immobilization, single cell culture, etc., as well as for improving other varieties of mango.

Mature raw fruits of mango used in the present invention are collected from Dapoli, Deogad and Vengurle.

In an embodiment, the present invention provides a primer sequence for amplifying enone oxidoreductase derived from mango selected from sequence having Seq. ID Nos. 1 -13.

In embodiment, the present invention discloses the complete open reading frame encoding enone oxidoreductase derived from mango as shown in Figure 1.

Accordingly, the novel isolated nucleotide sequence encoding enone oxidoreductase comprises the sequence ID No. 14.

In an embodiment, the present invention provides forward and reverse degenerate primers for enone oxidoreductase for amplification of the cDNA prepared from ripe fruits of mango.

The degenerate primers (Seq. ID No. 1 -7) designed for amplification of the mango cDNA are:

Forward 1 GTKGTKGCTGCWKCYVTTAAYC (Seq ID NO. 1)

Forward2 AARGMYAYYGAYTCTCCYYTRC (Seq ID NO. 2)

Forward3 GGVWSWTTRGCWGARTAYACHGC (Seq ID NO. 3)

Forward4 GTTYTRRRWGGHGCTGGKGGWGTTGG (Seq ID NO. 4)

Reverse 1 GRATSGGRTA YAYRACYACYTTYCC (Seq ID NO. 5)

Reverse2 GCYYTHTCHSKYTSYCCWAYTGC (Seq ID NO. 6)

Reverse3 RGTRGCTGCTAYYTTDGAWGCACC (Seq ID NO. 7) In another embodiment, the present invention provides forward and reverse gene specific primers for enone oxidoreductase for amplification of the ends of cDNA by rapid amplification of cDNA ends (RACE).

The gene specific primers (Seq ID NO. 8-1 1) designed for amplification of the ends of mango cDNA are:

Forward 1 CGAAGACAGGGCAAGTTCAAGGC (Seq ID NO. 8)

Forward2 GGTGTTGGAAGCTTGGTGATTCAG (Seq ID NO. 9)

Reverse 1 GATTCTCCCCTCCCGACTGTTCC (Seq ID NO. 10)

Reverse2 GGGTTCTCTGCTGGTAAATCTATTCT (Seq ID NO. 1 1 )

In yet another embodiment, the current invention provides primers corresponding to the terminal regions of the mRNA which are designed for enone oxidoreductase. These terminal primers are used for the PCR amplification with mango cDNA as a template.

The terminal primers (Seq. ID NO. 12 and 13) designed for the PCR amplification are:

Forward ATGAAAGCGTGGGTGTATGGAG (Seq ID NO. 12)

Reverse TTAAGGAATTGGGTATATAACCACC (Seq ID NO. 13)

The present invention further provides the process of isolating full-length nucleotide sequence (Seq ID no. 14) encoding enone oxidoreductase from ripe mangoes designated as EO. The process includes the following steps:

i. isolating RNA by CTAB method;

ii. treating total RNA with DNase and carrying out reverse transcription to obtain cDNA;

iii. designing degenerate primers for enone oxidoreductase based ori the alignment of data base entries reported in the NCBI database;

iv. amplifying cDNA of step (ii) using the degenerate primers; v. designing gene specific primers for enone oxidoreductase based on the sequence of the fragments obtained in step (iv);

vi. amplifying the ends of the cDNA using gene specific primers of step (v) by Rapid Amplification of cDNA Ends (RACE);

vii. designing primers corresponding to the terminal regions of mRNA based on the alignment of 5' and 3 ' RACE fragments with the enone oxidoreductase sequences reported from other plants; and

viii. amplifying mango cDNA using primers designed in step (vii) by PCR (polymerase chain reaction) to obtain a full length cDNA of a putative mango enone oxidoreductase.

The process of isolating full-length sequence of enone oxidoreductase from ripe mangoes comprises isolation of RNA by CTAB method. After treating isolated RNA with DNase, reverse transcription is carried out. Based on the conserved regions in the nucleotide sequences of orthologous enone oxidoreductase (EO) reported in the NCBI database, designated as quinone oxidoreductases from Fragaria x ananassa (AY048861), Vigna radiate (U20808) and Helianthus annuus (AF384244), degenerate primers are designed. These primers are used for the amplification of cDNA prepared from ripe fruits of mango. This is followed by designing gene specific primers based on the sequence of the fragments obtained by amplification over the cDNA. The gene specific primers are used for amplification of the ends of the cDNA by rapid amplification of cDNA ends (RACE). Based on the alignments of the 5' and 3' RACE fragments with the respective sequences reported from the other plants, primers corresponding to the terminal regions of the mRNA are designed and are used for obtaining full-length sequence of EO.

The degenerate primers designed in step (iii) of the process of isolating full-length nucleotide sequence encoding enone oxidoreductase from ripe mangoes are as follows;

Forward 1 GTKGTKGCTGCWKCYVTTAAYC

Forward2 AARGMYAYYGAYTCTCCYYTRC Forwarctf GGVWSWTTRGCWGARTAYACHGC

Forward4 GTTYTRRRWGGHGCTGGKGGWGTTGG

Reverse 1 GRATSGGRTAYAYRACYACYTTYCC

Reverse2 GCYYTHTCHSKYTSYCCWAYTGC

Reverse3 RGTRGCTGCTAYYTTDGAWGCACC

The gene specific primers designed in step (v) of the process of isolating full-length nucleotide sequence encoding enone oxidoreductase from ripe mangoes are as follows;

Forward 1 CGAAGACAGGGCAAGTTCAAGGC

Reverse 1 GATTCTCCCCTCCCGACTGTTCC

Forward2 GGTGTTGGAAGCTTGGTGATTCAG

Reverse2 GGGTTCTCTGCTGGTAAATCTATTCT

The terminal primers designed in step (vii) of the process of isolating full-length nucleotide sequence encoding enone oxidoreductase from ripe mangoes are as follows;

Forward ATGAAAGCGTGGGTGTATGGAG

Reverse TTAAGGAATTGGGTATATAACCACC

The complete open reading frame (ORF) of MiEO (Sequence ID No. 14) thus obtained is 1 143 base pair long and is flanked by a 40 base pair UTR at the 5' end and by a 1 15 base pair UTR at the 3' end. The ORF encodes a protein having 381 amino acids, a calculated molecular weight of 40.6 kD and a pi of 8.61.

In another embodiment, the present invention studies the actual role of MiEO in forming the profiles of furanones observed during the ripening of mango fruit, where the transcripts of MiEO are profiled through various ripening stages. The highest expression of MEO is detected at the 10 DAH (days after harvest) stage of the ripening fruits while a reduction in the expression of MiEO during the transition from 10 DAH to 15 DAH is observed. Since ripe mango fruits contain high amounts of the furanones, furaneol and mesifuran, and since MiEO produces furaneol in in vitro assays, it is observed that the most likely in planta function of MiEO is the biosynthesis of furaneol.

Accordingly, in the ripening fruits of mango, the peak level of furanones is detected at the ripe stage (15 DAH); whereas, the highest expression of MiEO is seen at 10 DAH stage. This discrepancy can be attributed to the fact that peak transcript level and synthesis usually precedes the highest accumulation of a substance. However, in strawberry it has been shown that the expression of a similar gene, FaEO, is highly correlated with the furanone levels during fruit development. Several reasons can be given for the differences between strawberry and mango. Most importantly, strawberry is a non-climacteric fruit and mango a climacteric fruit and so there are notable differences in the ripening physiology of these two fruits and in the expression of various genes. Secondly, the level of furanones observed in mango is about 5 fold lower than in strawberry, while the precursor of furaneol, HMMF, is not detected in the mango fruits. The lack of a strong correlation between MiEO expression and furanone accumulation points towards involvement of MiEO in functions in addition to the biosynthesis of furaneol.

In another embodiment, the present invention studies the similarity of the in silico translated amino acid sequence of MiEO with enzymes from other plants. The similarity of the in silico translated amino acid sequence of. MiEO is 79% with the chloroplastic alkenal/one oxidoreductase (AOR) from Cucumissativus (CsAOR), 73% with the enone oxidoreductase (EO) from Solanumlycopersicon (S1EO), 72% with the EO. from Fragaria x ananassa (FaEO) and 71% with the AOR from Arabidopsis thaliana (AtAOR). One such enzyme, CsAOR from Cucumissativus, which shows 79% sequence identity with MiEO, catalyses the reduction of α, β- unsaturated alkenals /alkenones in in vitro reactions. Similar oxidoreductase activity was also shown to be associated with an enzyme from Arabidopsis (AtAOR). The unsaturated aldehyde and ketone substrates of AORs, generated by lipid peroxidation, are highly reactive chemicals that can damage cellular activities by reacting with various biomolecules. Enzymes such as CsAOR and AtAOR are thought to be important for maintaining cellular processes by converting these harmful carbonyls into their saturated derivatives.

The analysis of the putative amino acid sequence of ΜΈΟ, strongly suggests that this protein might be localized in chloroplasts. This prediction can also be supported by the fact that chloroplasts are rich in fructose- 1, 6-diphosphate, the starting substrate for furaneol biosynthesis, which is produced by various pathways. Chloroplasts are also a center for production of highly reactive chemicals because of the high metabolic activity of this organelle, which can mainly be attributed to the process of photosynthesis and associated reactions. The increased rate of chemical reactions in chloroplasts of the fruits also results from the physiological transition of these organelles into chromoplasts, a most remarkable feature of fruit ripening. This conversion is characterized by various cellular changes such as dismantling of the thylakoid membrane system, which is brought about by degradation of its membrane lipids and chlorophylls, biosynthesis of carotenoids, and reduction in the amount of the proteins involved in photosynthesis. Some of these metabolic processes, especially the degradation of membrane lipids, are known to yield highly reactive compounds such as unsaturated carbonyls and reactive oxygen species. Since the chloroplast-located enzymes from the other plants, CsAOR and AtAOR, which are highly similar to Mz^'EO have been shown to be involved in scavenging of the reactive compounds, it is possible that MEO also might be involved in such processes instead of or in addition to the biosynthesis of furaneol. This hypothesis is supported by the fact that HMMF, the precursor of furaneol, is not detected in mango fruits. This observation along with the report of EO-like transcripts in the plants which have till now not been reported to contain furaneol (Table 1), and the absence of correlation between the transcript abundance of Mz^'EO and the level of furanones in the mango fruits might be taken to support an alternative function of Mz^'EO and a different biosynthetic pathway to the furanones. Table 1

Uncharacterized sequences from the NCBI database showing high identity with

MiEO

Accession number Plant Putative annotation Sequence identi with MiEO

XP 002525379 Ricinus communis Alcohol dehydrogenase 94 %

ABK96279 Populus trichocarpa x Unknown 90%

Populus deltoides

XP_002323668 Populus trichocarpa Unknown 90%

ADN33837 Cucumis melo Alcohol dehydrogenase 89%

Industrial advantages

Furaneoi and mesifuran are the two important ripening-related flavor chemicals of Alphonso mango. Biosynthesis of furaneoi is catalyzed by enone oxidoreductase which has been isolated from the Alphonso mango fruits in this study. Mango is only the third plant after strawberry and tomato from which such gene has been isolated and characterized. This coding sequences can be used for biotechnological production of the recombinant enone oxidoreductase enzyme which can be used for the production of furaneoi. The degenerate primers described here have been designed by homology-based approach based on the putative gene sequences reported from the other plants. These primers can thus be used for isolating similar genes from the other plants also. Similar work is being attempted by the Inventors in case of Alphonso mango as well as other economically important fruits and crops.

The novel nucleotide sequences of the present invention can be used for enzyme production in an artificial system and later this artificially synthesized enzyme can be mixed appropriately with any desired food product for generating the desired flavor. The nucleotide sequences can also be used for semi-biosynthesis of flavors via various approaches such as enzyme immobilization, single cell culture, etc., as well as to improve other varieties of mango. Also furaneoi, the product of mango enone oxidoreductase, is an important flavor compound, which has huge application in the food industry. References cited in the specification

Cruz-Hernandez A, Gomez-Lim MA. (1995). Alternative oxidase from mango (Mangifera indica, L.) is differentially regulated during fruit ripening. Planta.;197(4):569-76.

Klein, D., Fink, B., Arold, B., Eisenreich, W. & Schwab, W. (2007). Functional characterization of enone oxidoreductases from strawberry and tomato fruit. Journal of Agricultural and Food Chemistry 55, 6705-671 1.

Pandit, S. S., Kulkarni, R. S., Giri, A. P., Koellner, T. G., Degenhardt, J., Gershenzon, J. & Gupta, V. S. (2010). Expression profiling of various genes during the fruit development and ripening of mango. Plant Physiology and

Biochemistry (Paris) 48, 426-433.

Reddy, Y.V., Srivastava, G.C., (2001) Ethylene biosynthesis and respiration during ripening in mango cultivars. Indian Journal of Plant Physiology. 6, 361 -364.

EXAMPLES

The following examples are given by way of illustration and therefore should not be construed to limit the scope of the present invention.

EXAMPLE 1

Plant material

Mature raw fruits of mango were collected from the orchards of Konkan Krishi Vidyapeeth at Dapoli (Ν 17°45' E73°l Γ) and Deogad (Ν16°3 Γ Ε73°20') and from a private orchard at Vengurle (Ν15°5 Γ Ε73°39'). For each of the three localities, fruits were collected from four plants. After harvesting, fruits were put in the hay, carried to the laboratory and allowed to ripe at ambient temperature. At the interval of every five days, fruits were peeled, pulp was immediately frozen in the liquid nitrogen and stored at -80°C until use. Thus, the experimental tissues of four ripening stages: 0, 5, 10 and 15 DAH (days after harvest) were obtained from each of the three localities. RNA isolation and cDNA synthesis

RNA was isolated by CTAB method. After treating total RNA with DNase, reverse transcription was carried out over ^g of total RNA using Enhanced Avian RT First Strand Synthesis Kit (Sigma, St. Louis, MO, USA).

Based on the conserved regions in the nucleotide sequences of orthologous enone oxidoreductase (EO) reported in the NCBI database, degenerate primers were designed. These primers were used for the amplification over the cDNA prepared from ripe mango fruits. The gene specific primers designed based on the sequence of the fragments obtained were used for amplification of the ends of the cDNA by rapid amplification of cDNA ends (RACE) using a RACE kit (Clontech, USA). Based on the alignments of the 5' and 3' RACE fragments with the respective sequences reported from the other plants, primers corresponding to the terminal regions of the mRNA were designed and were used for the obtaining full-length sequence of Mangifera indica enone oxidoreductase (ΜΈΟ).

The complete open reading frame (ORF) of /ΈΟ thus obtained is 1 143 base pair long (Figure 1) and is flanked by a 40 base pair UTR at the 5' end and by a 1 15 base pair UTR at the 3' end. The ORF encodes a protein having 381 amino acids, a calculated molecular weight of 40.6 kD and a pi of 8.61.

The in silico translated sequence of EO was alignment with the closest characterized sequences from other plants. The putative amino acid sequence of MEO shows the presence of the conserved GxGxxG domain which is involved in binding with NADP. As shown in Figure 2, regions of the alignment corresponding to the nucleotide sequence used for designing degenerate primers are marked by the line below the alignment, and that used for designing gene specific primers for RACE is indicated by double lines above the alignment. The conserved NAD(P)H- binding domain is highlighted in the grey color. The arrow head indicates the truncation site for removing the putative chloroplast targeting sequence.

Similar to CsAOR, AtAOR and S1EO, the N-terminal region of the in silico translated MEO was characterized by the presence of putative chloroplast targeting peptide as revealed by analysis of the sequence by ChloroP program, suggesting that the EO protein might be localized in the chloroplast, as was shown for CsAOR.

EXAMPLE 2

Expression cloning and recombinant expression in E. coli

Full length sequence of EO was amplified using Expand High Fidelity PCR System (La Roche, Basel, Switzerland) with the terminal primers. cDNA prepared from the ripe fruit was used as the template and the resulting fragments of /ΈΟ was cloned in the pCRT7-NT/TOPO expression vector (Invitrogen). Ligation reaction was transformed in the E. coli cells (Topi OF', Invitrogen) and the transformants were selected on the LB-agar medium containing 100 μg/ml carbenicillin. The correct orientation of insert was confirmed by carrying out a PCR using forward T7 promoter primer and reverse gene specific primer, as well as by sequencing. The recombinant plasmids was transformed in BL21 (DE3) (Invitrogen) cells for recombinant expression. Starter culture (5 ml) grown for 48 hour at 18 °C in LB media was used as inoculum for the expression in 100 ml media with the Overnight Express Autoinduction System 1 ( ovagen, USA). Cultures were grown for 24 hour at 18°C and the pellet obtained after centrifugation was suspended in the buffer containing 25 miVI OPSO (pH 7.2) and 10% (v/v) glycerol. The cells were lysed by sonication and the (his)₆-tagged recombinant proteins were purified by passing the cleared lysate through Ni-NTA spin columns (Qiagen, Germany). Elution was carried out with the buffer containing 250 mM imidazole, 25 mM MOPSO (pH 7.2) and 10% (v/v) glycerol. Both crude lysate and the purified protein were checked for the presence and size determination of the recombinant protein by SDS-PAGE (Sambrook and Russell, 2001).

EXAMPLE 3

Assay for the enzymatic activity

Purified protein was incubated overnight at 30°C with 60 mg fructose- 1 , 6- diphosphate and 3 mg NADH in 1 ml buffer containing 25 mM MOPSO and 10% glycerol (pH 7). The products formed were purified by solid phase extraction (SPE) using the DSC- 18 columns having the capacity of 3 ml (Sigma, USA). The SPE column was first equilibrated with acetonitrile, followed by the assay buffer. After passing the incubation mixture, the products were eluted from the column with the help of dichloromethane and were analyzed by GC-MS. The product separation was carried out on the GsBP-5MS column having the dimensions of 30 m x 0.32 mm i.d. x 0.25 μιη film thickness (General Separation Technologies, USA). Oven temperatures were programmed from 40°C for 5 min, raised to 220°C at 10°C min- 1 and held isothermal for 5 min. Injector and detector temperatures were 150 and 250°C, respectively. Helium was used as carrier gas at a flow rate 1 ml min-1. Mass spectra were obtained using Clarus 500 (Perkin Elmer) gas chromatograph-mass spectrometer at 70 eV with a scan time of 0.2 s. To enhance the selectivity of the detection, only the ion of m/z 128 of furaneol was monitored. In the separate analysis total ion chromatograph was also recorded and was used for examining the spectra of the furaneol formed in the test assays.

Furaneol was detected in assays with the protein expressed from the plasmid having the reverse-oriented insert indicating that this activity is due to background proteins from the E. coli expression system. However, increasing the stringency of the wash solution to 40 mM imidazole during the purification of protein by affinity ' chromatography using Ni-NTA agarose spin columns resulted in diminishing of the oxidoreductase activity originating from E. coli.

The MEO protein purified and assayed with fructose- 1, 6-diphosphate clearly showed the presence of furaneol as a reaction product in the GC-MS analysis (Fig. 3 - a, b, c, d, e).

Although fructose-1, 6-diphosphate is not a direct natural precursor of furaneol, the enzyme from strawberry, FaEO was also shown to be able to covert fructose- 1,6- diphosphate to furaneol via an intermediate, HMMF. The detection of furaneol in assays of purified /ΈΟ with fructose-1, 6-diphosphate as substrate combined with the absence of furaneol in the assays of boiled protein thus confirmed the furaneol forming activity of MEO. EXAMPLE 4

Quantitative PCR analysis

Quantitative PCR was performed with Brilliant SYBR Green QPCR Master Mix (Stratagene, USA) with elongation factor la (EFla) as a normalizing gene. Primers used for amplifying a fragment of M/EO were: (forward) 5'- AGGTGCTGTAAC ACCTCCAGGCT-3 ' and (reverse) 5'-

CCTGGCTGAAAGG A AATGGCCCC-3 ' . Transcript abundance was quantified with a Mx3000P Real Time PCR Thermocycler (Stratagene) using a program with 45 cycles of 95°C for 30 seconds, 63°C for 30 secondsand 72°C for 30 seconds, followed by a melting curve analysis of transcripts. The relative transcript abundance of the raw stage (0 DAH) of mango was considered and the fold difference for the rest of the tissues was calculated. Each measurement was repeated with four independent biological replicates, each of which was represented by at least two technical replicates. Ripening stages were compared to each other for the relative transcript abundance of each of the genes between the ripening stages and localities by ANOVA with the aid of Fisher's LSD at p < 0.05 using StatView software, version 5.0 (SAS Institute Inc., USA).

The highest expression of MEO was detected at the 10 DAH (days after harvest) stage of the ripening fruits (Fig. 4). As can be seen in figure 4, the relative transcript abundance of M/EO for the raw stage (0 DAH) from Dapoli was considered 1 and the fold difference for the rest of the tissues was calculated. There was a reduction in the expression of M EO during the transition from 10 DAH to 15 DAH (ripe) fruits. Although furaneol and mesifuran are completely absent in the raw fruits (0 DAH), the expression level of MiEO was only about 1.5-fold lower than in the ripe fruits. There was about two fold reduction in expression during the transition of fruit from 0 to 5 DAH stage. Out of the three localities which were studied for the content of volatiles, Dapoli was characterized by the lowest amount of mesifuran in the ripe fruits; whereas, for the 10 DAH stage, the highest amount of mesifuran was detected in the fruits from Deogad. To know if there is any contribution of M/EO to such geographic variation, expression of M/EO was also analyzed in the ripening fruits of mangoes from these cultivation locations. Although there were some differences between the localities for the level of MiEO transcripts, the pattern could not be correlated with the varied mesifuran content among the localities.

Claims

We Claim:

1. A primer sequence selected from the group consisting of Seq. ID. Nos. 1-13 for amplifying enone oxidoreductase from mango.

An isolated novel nucleotide sequence encoding enone oxidoreductase from Mango comprising Seq. ID No. 14.

Use of Sequence ID No. 14 obtained by using primer sequence as claimed in claim 1, for semi-biosynthesis of flavors.

Use of Sequence ID No. 14 obtained by using primer sequence as claimed in claim 1 , for biosynthesis of furaneol in mango.

5. Use of Sequence ID No. 14 obtained by using primer sequence as claimed in claim 1, for enzyme production in an artificial system.

Use of Sequence ID No. 14 obtained by using primer sequence as claimed claim 1 , for improving mango varieties.