Allium fistulosum leaf agglutinin recombinant protein, its encoding polynucleotide, primer and process for preparation thereof

Abstract

Nucleic acid sequence encoding Allium fistulosum leaf agglutinin (AFAL) is disclosed. The invention provides Allium fistulosum leaf agglutinin (AFAL) recombinant protein, its encoding nucleotides, primers and the process of preparation thereof, said recombinant protein is useful for insect control and haemagglutination activity. AFAL is found more toxic to sap sucking insect pest Aphis gossypii (cotton aphid) and Bemisia tabaci (whiteflies) as compared to known Allium sativum leaf agglutinin. AFAL can be used in the development of transgenic plants for resistance against sap sucking and chewing pests.

Description

PRIORITY APPLICATIONS

This application is a U.S. National Stage Filing under 35 U.S.C. 371 from International Application No. PCT/IN2012/000822, filed on 17 Dec. 2012, and published as WO2013098852 on 4 Jul. 2013, which claims the benefit to Indian Application No. 3850/DEL/2011, filed on 28 Dec. 2011; which applications and publication are incorporated herein by reference in their entirety.

FIELD OF THE INVENTION

The invention relates to Allium fistulosum leaf agglutinin (AFAL) recombinant protein, its encoding polynucleotide, primers and process of preparation thereof said Allium fistulosum leaf agglutinin (AFAL) protein is useful for insecticidal activity and haemagglutination activity. In particular the present invention relates to nucleic acid sequence (afal) encoding for Allium fistulosum leaf agglutinin (AFAL) applicable for haemagglutination and insect control.

BACKGROUND AND PRIOR ART OF THE INVENTION

Plant lectins, also known as “agglutinins”, are heterogeneous group of carbohydrate binding proteins, which are able to bind simple sugars and/or complex carbohydrates reversibly (Van Damme et al. 1998; CRC Crit Rev Plant Sci 17:575-692). They show a marked heterogeneity with respect to their molecular structures, sugar binding specificity and temporal and spatial regulation. Mannose binding lectins are widely found in higher plants and play a significant role in defense due to their ability to recognize high-Mannose-type glycans of microbial pathogens and plant predators (Van Damme et al. 1998, 1998, CRC Grit Rev Plant Sci 17:575-692; Van Damme et al. 2004 Trends Plant Sci 9:484-9). Mannose binding lectin from garlic leaf [Allium sativum leaf agglutinin (ASAL)] is a 25 kDa homodimeric protein, structurally and evolutionarily related to Galanthus nivalis agglutinin (GNA) (Smeets et al. 1997a, Plant Mol Biol 35: 531-535; Van Damme et al. 1992, Eur J Biochem 206:413-420). Some of the biological properties of ASAL are—(1) it readily agglutinates rabbit erythrocytes but does not affect human erythrocytes (Bandhopadhyay et. al. 2001, Plant Sci. 161:1025-1033; Smeets et al. 1997a, Plant Mol Biol 35: 531-535), (2) it has inhibitory effect against retrovirus (HIV1 and HIV2) induced cytopathicity in MT-4 cells (Smeets et. al. 1997b, Plant Mol Biol 33:223-234) and (3) it is toxic (growth inhibitory) against a spectrum of insects of order Homoptera, Lepidoptera and Coleoptera. Some important pests inhibited by ASAL are aphids [mustard aphid, peach potato aphid, tobacco aphid (Bandhopadhyay et al. 2001, Plant Mol Biol 33:223-234 Hossain et al. 2006, Crop Sci 46:2022-2032; Smeets et al. 1997a, Plant Mol Biol 35: 531-535), red cotton bug (Bandhopadhyay et al. 2001, Plant. Mol. Biol. 33:223-234), brown plant hopper, green leaf hopper (Saha et al. 2006, Plant Mol. Biol. 62:735-52) and cotton leaf worm (Sadeghi et al. 2008, Transgenic Res. 17:9-18). Although exact mechanism of insecticidal action of lectins is still not well understood, three different modes of action have been proposed—(1) binding of the lectins to the peritrophic matrix of the midgut, inhibiting nutrient absorption (Harper et al 1998, Tissue Cell 30: 166-176), (2) binding to glycoproteins on epithelial cells of the midgut and disrupting tissue integrity (Powell et al. 1998, J Insect Physiol. 44: 529-539; Sauvion et al. 2004, J Insect Physiol. 50: 1137-1150) and (3) binding to carbohydrate moieties of the sensory receptors of insect mouth parts, disrupting membrane integrity and interfering in the food detection ability of insects (Murdock et al. 2002, J Agric Food Chem. 50: 6605-6611). All these mechanisms result in decreased ability of insect to ingest food or absorb nutrients, leading to delayed development and premature death.

U.S. Pat. No. 5,545,820 (Gatehouse, et al., 1996) discloses the use of lectins having specific mannose-binding ability, derived from family Amaryllidaceae or Alliaceae for the control of insect pests. WO/1992/002139 relates to the use of lectins having specific mannose-binding ability, derived from family Amaryllidaceae or Alliaceae for the control of insect pests and the development of transgenic plants expressing such lectins. U.S. Pat. No. 5,407,454 relates to selected plant lectins having larvicidal activity against a number of common insect pests of agricultural crops. Insect resistance in the transgenic plants is due to insertion of larvicidal lectin gene in all the cells of the plants.

U.S. Pat. No. 6,127,532 (Raikhel) refers to transgenic plants containing cDNA encoding Gramineae lectin. Such transgenic plants expressed barley lectin and stored in in the leaves. The transgenic plants, particularly the leaves exhibit insecticidal and fungicidal′ properties.

Allium fistulosum

Allium fistulosum L. (Welsh onion, Japanese bunching onion) is a perennial onion. Other names that may apply to this plant include green onion, spring onion, escallion, and salad onion. These names are ambiguous, as they may also be used to refer to any young green onion stalk, whether grown from Welsh onions, common bulb onions, or other similar members of the genus Allium. The species is very similar in taste and odor to the related bulb onion, Allium cepa, and hybrids between the two (tree onions). The Welsh onion, however, does not develop bulbs, and possesses hollow leaves (“fistulosum” means “hollow”) and scapes. Large varieties of the Welsh onion resemble the leek, such as the Japanese ‘negi’, whilst smaller varieties resemble chives. Many Welsh onions can be multiplied by forming perennial evergreen clumps. Next to culinary use, it is also grown as an ornamental plant. Historically, the Welsh onion was known as the cibol.

The name “Welsh onion” has become a misnomer in modern English, as Allium fistulosum is not indigenous to Wales. “Welsh” preserves the original meaning of the Old English word “welisc”, or Old German “welsche”, meaning “foreign” (compare wal- in “walnut”, of the same etymological origin). The species originated in Asia, possibly Siberia or China.

Culinary Use

In the West, the Welsh onion is primarily used as a scallion or salad onion, but is widely used in other parts of the world, particularly East Asia.

• Russia: Welsh onion is used in Russia in the spring for adding green leaves to salads.
• Asia: The Welsh onion is an ingredient in Asian cuisine, especially in East and Southeast Asia. It is particularly important in China, Japan, and Korea, hence the other English name for this plant, ‘Japanese bunching onion’. Bulb onions were introduced to East Asia in the 19th century, but A. fistulosum remains more popular and widespread. In Japan, it is used in miso soup, negimaki (beef and scallion rolls), among others, and it is widely sliced up and used as a garnish on teriyaki or takoyaki.
• Jamaica: Known as escallion, the Welsh onion is an ingredient in Jamaican cuisine, in combination with thyme, scotch bonnet pepper, garlic and allspice (called pimenta). Recipes with escallion sometimes suggest leek as a substitute in salads. Jamaican dried spice mixtures using escallion are available commercially. The Jamaican name is probably a variant of scallion, the term used loosely for the spring onion and various other plants in the genus Allium. Lacking in the Prior Art

Allium lectin disclosed in present invention shows high insecticidal activity and therefore novel. Homology of the nucleotide sequence with available nucleotide sequences in database shows more than 90% homology.

OBJECTIVES OF THE INVENTION

• • a) The main objective of the invention is to provide nucleic acid sequence which encodes for Allium fistulosum leaf agglutinin
  • b) Another objective of the present invention is to provide gene specific primers

SEQ ID NO: 5
GSP 1 (5′-ATGGACAGTACTCCATCTCCTAAAC-3′);
and
SEQ ID NO: 6
GSP 2 (5′-TTAGCCCCTTGGCCTCCTGCA-3′),

• •  useful for amplification of the gene.
  • c) Another objective of the present invention is to provide agglutinin recombinant protein having high insecticidal activity
  • d) Another objective of the present invention is the application of Allium fistulosum leaf agglutinin protein for insect control.

SUMMARY OF THE INVENTION

Accordingly, the present invention relates to Allium fistulosum leaf agglutinin (AFAL) recombinant protein, its encoding nucleotides, primers and the process of preparation thereof, said protein is useful for insect control and haemagglutination activity.

In an embodiment of present invention, the process of preparation of Allium fistulosum leaf agglutinin (afal) recombinant protein, useful for insecticidal activity and haemagglutination activity, comprising of following steps—

• • a) Extracting of total RNA from the Allium fistulosum leaves
  • b) Synthesizing of cDNA from total RNA extracted from leaves of Allium fistulosum
  • c) Designing of primers GSP1 and GSP2 from 5′- and 3′-RACE fragment of c DNA to clone full-length protein encoding DNA, designing of primers GSP3 and GSP4 for cloning of the DNA encoding mature polypeptide of AFAL protein,
  • d) Expressing the DNA encoding the mature AFAL in E. coli SUMO expression vector where SUMO peptide is fused with AFAL at the N-terminus and expressed in E. coli under T7 promoter to get desired AFAL recombinant protein.

In another embodiment of the present invention the primers GSP1 and GSP2 comprise:

• • 1. GSP1 represented by SEQ ID NO:5, and
  • 2. GSP2 represented by SEQ ID NO:6.

Allium fistulosum leaf agglutinin (AFAL) recombinant protein is 8-10 fold more toxic to cotton aphid (Aphis gossypii) and 6-8 fold to whiteflies (Bemisia tabaci) as compared to well-known Allium sativum leaf agglutinin.

According to the invention a DNA fragment of 651 bp was cloned from total cDNA of A. fistulosum leaves, consisted of, 585 bp long open reading frame encoding AFAL precursor protein of 194 amino acid residues with 28 amino acid long N-terminal signal peptide and 56 amino acid long C-terminal peptide. The amino acid sequences of AFAL are different from the other reported Allium lectin sequences. The cloned genomic DNA sequence of afal showed absence of intron.

In another embodiment of the present invention the nucleic acid sequence having SEQ ID NO:2, encodes a polypeptide as represented in SEQ ID NO:4, which is a 110 amino acid residue long mature peptide ofAllium fistulosum leaf agglutinin(AFAL), having a molecular weight of ˜12 kDa.

In yet another embodiment of the present invention the polypeptide has the minimum haemagglutination value of in the range of 6-10 ng/ml.

In yet another embodiment of the present invention the polypeptide exhibits insecticidal activity selected from the group comprising haemagglutination, insecticidal, antifungal and anti-prolific activity.

In still yet another embodiment of the present invention the polypeptide exhibits haemagglutination activity selected from the group comprising haemagglutination, insecticidal, antifungal and anti-prolific activity.

BRIEF DESCRIPTION OF FIGURES

FIG. 1A. Lane 1, Molecular weight markers; Lane 2, Total soluble protein from leaves of A. fistulosum; Lane 3, Unbound total soluble protein; Lane 4, Column wash (before elution); Lanes 5-8, eluted fractions. FIG. 1B. Lane 1, Molecular weight markers; Lane 2, Purified AFAL concentrated on 10 kDa cut-off filtration device.

FIG. 2. Peptide mass fingerprinting of AFAL

FIG. 3. V-bottom plate showing haemagglutination of rabbit erythrocytes by AFAL

FIG. 4 Clustalw analysis of AFAL with other Allium lectins. Amino acid identity of AFAL with other mannose binding lectins vary from 67% to 75%. Dark area represents mannose binding domain. (SEQ ID NOs: 3 and 12-17).

FIG. 5. Lane 1, Molecular weight markers; lane 2. uninduced bacterial lysate; lane 3-5, sample after 1 h, 2 h and 3 h induction; lane 6, supernatant of 3 hr induced culture; lane 7, protein in inclusion.

FIG. 6. Lane 1, molecular weight markers; lane 2, total E. coli protein containing SUMO-AFAL; lanes 3-4 represent purified fusion protein.

DETAILED DESCRIPTION OF THE INVENTION

The leaves of Allium fistulosum were collected from the National Bureau of Plant Genetic Resources, Bhowali, Nainital, Uttarakhand, India, and used for the purification of Allium fistulosum leaf agglutinin (AFAL). It was purified on mannose-agarose affinity column, followed by cut-off filtration device (Example 1, FIGS. 1 & 2). The purified protein was used for brief characterization.

AFAL shows several times better insecticidal activity against sap sucking pest Aphis gossypii (cotton aphids), Bemisia tabaci (whitefly) as compared to ASAL (Example 3). Large amount of purified protein is required for further characterization. The purification of AFAL from plant leaves in bulk amount is difficult due to unavailability of plant material and very low accumulation of the lectin in leaves. Expression of protein in a re combinant system is an alternative approach to produce the desired protein in large amount, which required the cloning of AFAL encoding gene. The gene (afal) was cloned from cDNA prepared from total RNA of leaves of A. fistulosum. The cloning was done by RACE (Rapid Amplification of cDNA Ends) using degenerate primers designed from the conserved mannose binding domain.

The cloned DNA fragment gene was of 651 bp, consisted of 585 bp open reading frame, 66 bp 5′ untranslated leader sequence. The full-length gene encoding AFAL precursor protein of 194 amino acid residues had 28 amino acid long N-terminal signal and 56 amino acid long C-terminal peptide. It contains three mannose binding domains as reported in the case of other mannose binding lectins (Example 5). The cloned genomic DNA sequence of afal had no intron. The amino acid sequences of AFAL are different from the other reported Allium lectin sequences (Example 5, FIG. 4).

The gene encoding insecticidal protein was cloned in E. coli expression vector in fusion with SUMO peptide and the recombinant insecticidal protein was expressed. The protein was purified on Ni-NTA column. The recombinant protein showed the insecticidal activity against cotton aphids and whiteflies. The gene encoding the mature peptide was cloned in plant expression vector pBI121 under CaMVE35S promoter (Example 6-8).

In the embodiment of the invention, the cloned full-length gene sequence of Allium fistulosum leaf agglutinin (afal) similar to SEQ ID NO:1. SEQ ID NO:1 contains DNA sequence which encodes N-terminal signal peptide, mature peptide and C-terminal peptide.

In another embodiment of the invention, nucleotides encoding N-terminal signal peptide and C-terminal peptide are removed from SEQ ID NO:1, to obtain the mature protein encoding gene sequence, similar to SEQ ID NO:2.

In another embodiment of the invention, the gene sequence of SEQ ID NO:1 was translated to obtain the full-length amino acid sequences of AFAL similar to SEQ ID NO:3.

In yet another embodiment of the invention, the gene sequence of SEQ ID NO:2 was translated to obtain mature AFAL with amino acid sequence similar to SEQ ID NO:4.

In yet another embodiment of the invention, the gene encoding the mature AFAL is cloned in E. coli SUMO expression vector where SUMO peptide is fused with AFAL at the N-terminus and expressed in E. coli under T7 promoter.

In yet another embodiment of the invention, the AFAL agglutinated rabbit erythrocytes.

In yet another embodiment of the invention, the AFAL was tested against insect pests like cotton aphid (Aphis gossypii) and whiteflies (Bemisia tabaci).

In yet another embodiment of the invention, the gene encoding the mature AFAL was cloned in plant expression vector under constitutive promoter CaMV35S and phloem specific promoters CoYMoV, RSS1, RolC etc. and expressed in transgenic plants for insect control.

(5) Examples

Example 1

Isolation and Purification of the Protein

Allium fistulosum leaves were collected from National Bureau of Plant Genetic Resources, Regional Centre, Bhawali, Uttaranchal, India. The protein was purified according to the protocol described (Smeets et al., 1997b). The purified protein was further purified on 50 kDa cut-off filtration device. The purified protein was concentrated on 10 kDa cut-off filter and stabilized in PBS for experiments.

Example 2

Peptide Mass Finger Printing

The purified protein was resolved on SDS-PAGE. The protein band was excised and digested with trypsin and used for peptide mass finger printing. The data was analyzed on MASCOT search. The peptides were found matching to the mannose binding lectins (FIG. 2).

Example 3

Haemagglutination Assay

Haemagglutination assays with rabbit RBCs were carried out in V-bottomed microtitre plates. Total volume of assay was 100 μl, 50 μl aliquot of two-fold serially diluted lectin in PBS was mixed with 50 μl 1 of 2% trypsinized rabbit erythrocytes suspension. Microtitre plate was incubated for 1 hour at room temperature. Agglutination was assessed visually. Reciprocal of the highest dilution of lectin showing detectable agglutination was taken as titer of the haemagglutination

TABLE 1
Haemagglutination assay of AFAL and its comparision with ASAL
S.N	Agglutinin	Haemagglutination
1	Allium sativum agglutinin (standard)	200 ng/ml
2	Allium fistulosum leaf agglutinin	8 ng/ml

Example 4

Insect Bioassay

Insect bioassay was carried out against sap sucking pest, cotton aphid (Aphis gossypii) and whiteflies (Bemisia tabaci). The known amount of purified protein was mixed in synthetic diet and insect mortality data was recorded at different time interval. The data was used for the calculation of LC₅₀ using probit analysis.

TABLE 2
Insecticidal activity of AFAL purified from leaves of A. fistulosum.
		Aphids	Whiteflies
		(Aphis gossypii),	(Bemisia tabaci),
S.N	Agglutinin	LC50	LC50
1	Allium sativum	68 μg/ml	76 μg/ml
	agglutinin (Standard)
2	Galanthus nivalis	51.39 μg/ml	53.39 μg/ml
	agglutinin
3	Allium fistulosum	7.1 μg/ml	8.5 μg/ml
	agglutinin

Example 5

Gene Cloning and Characterization

cDNA was synthesized following standard protocol. The 3′ RACE was performed with degenerate primer {5′ATGCA(A/G)(C/G)A (G/T)GACTGCAACC-3′; SEQ ID NO:11}(primer sequence was derived from the mannose-binding site, QXDXNXVXY (SEQ ID NO:10), conserved among most of the monocot mannose-binding lectins) and universal primer. For 5′ RACE, RNA was reversely transcribed with the 5′-RACE CDS Primer. Based on the 3′ and 5′ RACE results, primers were designed for amplification of full length gene, GSP1 (5′-ATGGACAGTACTCCATCTCCTAAAC-3′; SEQ ID NO:5) GSP2 (5′- GCCCCTTGGCCTCCTGCA-3′; SEQ ID NO:9). The full-length gene was amplified and cloned. The mature AFAL encoding DNA was amplified with primers

SEQ ID NO: 7
GSP 3 (5′-AGAAACGTATTGGTGAACAACG-3′);
and
SEQ ID NO: 8
GSP 4 (5′-TTATCTTCTGTAGGTACCAGTAGAC-3′).

The amino acid sequence of AFAL was deduced with Expasy translate tool. The analysis and comparison of the deduced amino acid sequences and nucleotide sequences obtained in RACE was performed with blast p (Standard Protein-Protein BLAST), blastn (Standard Nucleotide-Nucleotide BLAST) on NCBI (www.ncbi.nlm.nih.gov) and clustal W.

SEQ ID NO:1 Nucleic acid sequences encoding full-length AFAL

SEQ ID NO:2 Nucleic acid sequences encoding mature AFAL.

SEQ ID NO:3 Amino acid sequence of the Allium fistulosum leaf agglutinin

SEQ ID NO:4 Amino acid sequence of the mature Allium fistulosum leaf agglutinin

Nucleic acid sequences encoding full length AFAL
SEQ ID NO: 1
ATGGACAGTA CTCCATCTCC TAAACTAATG AGCATGACCA 60
CTGTAGCCAC CATCCTAACC
ATTTTGGCAT CTACATGCAT GGCCAGAAAC GTATTGGTGA 120
ACAACGAAGG ACTGTACGCA
GGCCAATCCC TAGTCGTAGA ACAGTACACT TTTACAATGC 180
AGGATGACTG CAACCTTGTA
CTCTACGAAT ACTGCGCCCC AATCTGGGCC TCAAACACGG 240
GCGTCACCGG CAAAAATGGG
TGCAGGGCCG TGATGCAGGC TGATGGCAAC TTTGTGGTCT 300
ACGATGTTAA CGGGCGTGCC
GTCTGGGCCA GTAACAGCAG AAGAGGGAAC GGAAACTATA 360
TCCTGGTGCT TCAGGAGGAC
AGGAACGTTG TTATTTACGG ATCTGATATT TGGTCTACTG 420
GTACGTACAG AAGAGGGCCC
GGTCCTGGTC CTGGTGCCGC CTGCAAGTGC GATGACGATG 480
GTCCTGACAT TCGCAGTGCT
ACTTTGACAG GCACTGTCGA TTTGGGAAGC TGCAACGAGG 540
GATGGGAGAA GTGCGCATCT
TTCTACACCA TCCTCGCGGA TTGCTGCAGG AGGCCAAGGG 585
GCTAA
Nucleic acid sequences encoding mature AFAL.
SEQ ID NO: 2
AGAAACGTAT TGGTGAACAA CGAAGGACTG TACGCAGGCC 60
AATCCCTAGT CGTAGAACAG
TACACTTTTA CAATGCAGGA TGACTGCAAC CTTGTACTCT 120
ACGAATACTG CGCCCCAATC
TGGGCCTCAA ACACGGGCGT CACCGGCAAA AATGGGTGCA 180
GGGCCGTGAT GCAGGCTGAT
GGCAACTTTG TGGTCTACGA TGTTAACGGG CGTGCCGTCT 240
GGGCCAGTAA CAGCAGAAGA
GGGAACGCAA ACTATATCCT GGTGCTTCAG GAGGACAGGA 300
ACGTTGTTAT TTACGGATCT
GATATTTGGT CTACTGGTAC GTACAGAAGA 330
Amino acid sequence of AFAL
SEQ ID NO: 3
MET ASP SER THR PRO SER PRO LYS LEU MET SER 20
MET THR THR VAL ALA THR ILE LEU THR
ILE LEU ALA SER THR CYS MET ALA ARG ASN VAL 40
LEU VAL ASN ASN GLU GLY LEU TYR ALA
GLY GLN SER LEU VAL VAL GLU GLN TYR THR PHE 60
THR MET GLN ASP ASP CYS ASN LEU VAL
LEU TYR GLU TYR CYS ALA PRO ILE TRP ALA SER 80
ASN THR GLY VAL THR GLY LYS ASN GLY
CYS ARG ALA VAL MET GLN ALA ASP GLY ASN PHE 100
VAL VAL TYR ASP VAL ASN GLY ARG ALA
VAL TRP ALA SER ASN SER ARG ARG GLY ASN GLY 120
ASN TYR ILE LEU VAL LEU GLN GLU ASP
ARG ASN VAL VAL ILE TYR GLY SER ASP ILE TRP 140
SER THR GLY THE TYR ARG ARG GLY PRO
GLY PRO GLY PRO GLY ALA ALA CYS LYS CYS ASP 160
ASP ASP GLY PRO ASP ILE ARG SER ALA
THR LEU THR GLY THE VAL ASP LEU GLY SER CYS 180
ASN GLU GLY TRP GLU LYS CYS ALA SER
PHE TYR THR ILE LEU ALA ASP CYS CYS ARG ARG 194
PRO ARG GLY
Amino acid sequence of the mature AFAL
SEQ ID NO: 4
ARG ASN VAL LEU VAL ASN ASN GLU GLY LEU TYR 20
ALA GLY GLN SER LEU VAL VAL GLU GLN
TYR THR PHE THR MET GLN ASP ASP CYS ASN LEU 40
VAL LEO TYR GLU TYR CYS ALA PRO ILE
TRP ALA SER ASN THR GLY VAL THR GLY LYS ASN 60
GLY CYS ARG ALA VAL MET GLN ALA ASP
GLY ASN PHE VAL VAL TYR ASP VAL ASN GLY ARG 80
ALA VAL TRP ALA SER ASN SER ARG ARG
GLY ASN GLY ASN TYR ILE LEU VAL LEU GLN GLU 100
ASP ARG ASN VAL VAL ILE TYR GLY SER
ASP ILE TRP SER THR GLY THR TYR ARG ARG 110
Primer sequence GSP1:
SEQ ID NO: 5
(5′-ATGGACAGTACTCCATCTCCTAAAC-3′).
Primer sequence GSP2:
SEQ ID NO: 6
(5′-GCCCCTTGGCCTCCTGCA-3′).
Primer sequence GSP3:
SEQ ID NO: 7
(5′-AGAAACGTATTGGTGAACAACG-3′).
Primer sequence GSP4:
SEQ ID NO: 8
(5′-TTATCTTCTGTAGGTACCAGTAGAC-3′)..

Example 6

Expression of AFAL with N-Terminal Fusion of SUMO in E. coli and Purification of SUMO-AFAL

The gene encoding mature AFAL was cloned in E. coli expression vector in fusion with SUMO peptide under T7 promoter. SUMO had (His₆) tag attached which helped in the purification of recombinantly expressed protein on Ni-NTA resin. SUMO-AFAL was expressed after induction with IPTG. The expression of the recombinant protein was observed every hour for 3 hours. After 3 hours of induction, cells were harvested by centrifugation; suspended in 20 mM TrisCl (pH 8). Bacterial cells were lysed by lysozymen and disrupted by sonication. The lysed bacterial cells were spun and supernatant and pellet were collected and electrophorased on denaturing PAGE (FIG. 5). Approximately half of the recombinant protein was in the soluble form and rest as inclusion in the pellet.

Purification of SUMO-AFAL from E. coli

Recombinantly expressed SUMO-AFAL was purified on metal-affinity column. Total bacterial protein was loaded on Ni-column, pre-equilibrated with the buffer (20 mM Tris pH 8, 300 mM NaCl and 10 mM Imidazole). NaCl and Imidazole were used to prevent the binding of non-specific proteins to the column. The column was washed with same buffer having 20 mM imidazole to remove low affinity bound proteins. Finally, the protein was eluted with 200 mM Imidazole (FIG. 6).

Example 7

Insect Bioassay with Recombinant Fusion Protein

Insect bioassay was carried out against sap sucking pest, cotton aphid (Aphis gossypii) and whiteflies (Bemisia tabaci). The known amount of SUMO-AFAL was mixed in synthetic diet and insect mortality data was recorded at different time interval. The data was used for the calculation of LC₅₀ using probit analysis. SUMO-ASAL served as positive control. The results of insect bioassay is shown in the table 3

TABLE 3
	LC50
			Whiteflies
S.N	Agglutinin	Aphids (Aphis gossypii)	(Bemisia tabaci)
1	Recombinant ASAL	55.05 μg/ml	51.2 μg/ml
	(SUMO-ASAL)
2	Recombinant AFAL	4.97 μg/ml	8.80 μg/ml
	(SUMO-AFAL)

Advantages of the Invention

The lectin protein being disclosed in the present invention (AFAL) is 6-10 folds more toxic to insects like aphids and whiteflies as compared to the standard Allium sativum leaf lectin (ASAL). AFAL also showed 25 folds higher haemagglutination activity as compared to ASAL. AFAL binds to lesser number of carbohydrate residues on glycans array as compared to ASAL. This assures fewer non-specific binding of AFAL to carbohydrates and therefore expected to be safe as compared to ASAL.

REFERENCES CITED

US patents
	5,545,820	Aug. 13, 1996	Gatehouse et al
	6,127,532	Oct. 3, 2000	Raikhel
	WO/1992/002139	Feb. 20, 1992	Gatehouse et al
	5,407,454	Apr. 18, 1995	Anthony et al

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Claims

1. A process for preparation of Allium fistulosum leaf agglutinin (AFAL) recombinant protein by amplifying the AFAL gene, wherein the process comprises: a) extracting total RNA from Allium fistulosum leaves;b) synthesizing cDNA from total RNA extracted from the leaves of Allium fistulosum; c) employing primers with a nucleotide sequence as set forth in SEQ ID NO:5 and SEQ ID NO:6 with cDNA of (b) to amplify and obtain a nucleotide fragment encoding full-length AFAL protein;d) employing primers having nucleotide sequences as set forth in SEQ ID NO:7 and SEQ ID NO:8 with said nucleotide fragment to amplify and obtain a polynucleotide fragment encoding mature AFAL protein;e) obtaining an expression cassette comprising said polynucleotide fragment and a promoter;f) introducing said expression cassette in a host to obtain recombinant host cells; andg) culturing said recombinant host cells to obtain recombinant AFAL protein.

2. Nucleic acid sequence represented by SEQ ID NO:1, obtained by the process claimed in claim 1, wherein SEQ ID NO:1 is comprised of 1 to 585 nucleotides or the sequence complementary thereto, which encodes full-length Allium fistulosum leaf agglutinin polypeptide, wherein nucleotide sequence 583 to 585 is a stop codon.

3. A cDNA fragment having a nucleic acid sequence as set forth in SEQ ID NO:2.

4. A method to express Allium fistulosum leaf agglutinin (AFAL) polypeptide, comprising: introducing to a cell genome a vector comprising a nucleotide sequence having SEQ ID NO:1 or SEQ ID NO:2 operably linked to a promoter expressed in E. coli, Pseudomonas, Pichia pastoris or Saccharomyces cerevisiae; and isolating from the cell a polypeptide having an amino acid sequence as set forth in SEQ ID NO:4, wherein the said polypeptide is a 110 amino acid residue long mature peptide of Allium fistulosum leaf agglutinin (AFAL) recombinant protein, having a molecular weight of about 12 kDa.

5. A method for making a plant resistant to insects, said method comprising producing an amount of isolated polypeptide having an amino acid sequence as set forth in SEQ ID NO: 4 in said plant, effective to exhibit insecticidal activity against the insect, wherein said plant is transformed with a nucleic acid having SEQ ID NO: 1.

6. The method as claimed in claim 5, wherein the isolated protein is in an amount that exhibits insecticidal activity against Aphis gossypii, Bemisia tabaci, Helicoverpa armigera and Spodoptera litura.

7. The method as claimed in claim 5, wherein the insect belongs to order lepidoptera, homoptera, coleopteran, or diptera.