Cloning and expression of coat protein gene of sweet potato leaf curl virus (splcv)
By: Sruthy, G S.
Contributor(s): Makeshkumar (Guide).
Material type:
BookPublisher: Vellayani Department of Plant Biotechnology, College of Agriculture 2018Description: 95p.Subject(s): Plant BiotechnologyDDC classification: 660.6 Online resources: Click here to access online Dissertation note: BSc-MSc (Integrated) Abstract: The study entitled “Cloning and expression of coat protein gene of sweet potato leaf curl
virus was carried out at the division of crop protection, Central Tuber Crops Research Institute,
Sreekariyam, Thiruvananthapuram during 2017-2018. The objective of the study was to clone
and express the coat protein gene of sweet potato leaf curl virus.
Sweet potato samples with Sweet potato leaf curl symptoms were
collected from the germplasm repository of ICAR-CTCRI Thiruvananthapuram and field
samples from regional station Bhuvaneshwar. Initial screening of Sweet potato leaf curl virus
was done with the specific partial coat protein primers which give the bands with the amplicon
size of 470bp. Out of 35 samples 10 samples were shows the SPLCV positive infection. Whole
genome amplification of Sweet potato leaf curl virus was done by rolling circle amplification
method. PBS2KS+ vector is used in the cloning purpose. Recombinant colonies were confirmed
by restriction analysis with BamHI. Sequencing was done by SPLCV specific primers PW285.2,
SPG1, SPG4, M13 R and T3. Sequences shows maximum similarity (90%) with Sweet potato
leaf curl Greece virus isolates (KF697069.1).
For the whole coat protein gene amplification new primers were designed by adding NdeI
and KpnI restriction digestion sites. Standardization of primer was done and kept melting
temperature at 55.9°C for further PCR amplification. Whole coat protein gene amplification was
done which give the bands at 776 bp. Eluted PCR products were cloned in PTZ57R/T vector and
transformed in to DH5α cells. Plasmids were isolated from recombinant colonies and
confirmation was done with restriction digestion with SacI and HindIII. Sequence analysis was
done for further studies which show 98% similarity with Sweet potato leaf curl virus CTCRI
isolate.
The recombinant PTZ57R/T vector is restricted with SacI and HindIII is eluted and
cloned into expression vectors such as pMALp5X, pET28a+ and pQE expression vectors.
SPLCV-CP insert concentration was high in pET28a+, hence further expression studies
pET28a+ was selected. The CP gene was cloned in pET 28a+ vector and transformed into BL21
cells. The BL21 clone containing the inframe CP gene was subjected to protein expression by
IPTG induction. The protein expression was optimum at 37°C for 3 h with an IPTG
concentration of l mM. The expressed protein showed a molecular weight of appropriate size of
32 kDa, when analysed on 12% SDS-PAGE. Expressed protein confirmed by Dot Immuno Blot
Assay (DIBA). This expressed protein can be used for the production of antiserum. These aids in
the serological detection of Sweet potato leaf curl virus infection.
| Item type | Current location | Collection | Call number | Status | Date due | Barcode |
|---|---|---|---|---|---|---|
Theses
|
KAU Central Library, Thrissur Theses | Reference Book | 660.6 SRU/CL (Browse shelf) | Not For Loan | 174416 |
BSc-MSc (Integrated)
The study entitled “Cloning and expression of coat protein gene of sweet potato leaf curl
virus was carried out at the division of crop protection, Central Tuber Crops Research Institute,
Sreekariyam, Thiruvananthapuram during 2017-2018. The objective of the study was to clone
and express the coat protein gene of sweet potato leaf curl virus.
Sweet potato samples with Sweet potato leaf curl symptoms were
collected from the germplasm repository of ICAR-CTCRI Thiruvananthapuram and field
samples from regional station Bhuvaneshwar. Initial screening of Sweet potato leaf curl virus
was done with the specific partial coat protein primers which give the bands with the amplicon
size of 470bp. Out of 35 samples 10 samples were shows the SPLCV positive infection. Whole
genome amplification of Sweet potato leaf curl virus was done by rolling circle amplification
method. PBS2KS+ vector is used in the cloning purpose. Recombinant colonies were confirmed
by restriction analysis with BamHI. Sequencing was done by SPLCV specific primers PW285.2,
SPG1, SPG4, M13 R and T3. Sequences shows maximum similarity (90%) with Sweet potato
leaf curl Greece virus isolates (KF697069.1).
For the whole coat protein gene amplification new primers were designed by adding NdeI
and KpnI restriction digestion sites. Standardization of primer was done and kept melting
temperature at 55.9°C for further PCR amplification. Whole coat protein gene amplification was
done which give the bands at 776 bp. Eluted PCR products were cloned in PTZ57R/T vector and
transformed in to DH5α cells. Plasmids were isolated from recombinant colonies and
confirmation was done with restriction digestion with SacI and HindIII. Sequence analysis was
done for further studies which show 98% similarity with Sweet potato leaf curl virus CTCRI
isolate.
The recombinant PTZ57R/T vector is restricted with SacI and HindIII is eluted and
cloned into expression vectors such as pMALp5X, pET28a+ and pQE expression vectors.
SPLCV-CP insert concentration was high in pET28a+, hence further expression studies
pET28a+ was selected. The CP gene was cloned in pET 28a+ vector and transformed into BL21
cells. The BL21 clone containing the inframe CP gene was subjected to protein expression by
IPTG induction. The protein expression was optimum at 37°C for 3 h with an IPTG
concentration of l mM. The expressed protein showed a molecular weight of appropriate size of
32 kDa, when analysed on 12% SDS-PAGE. Expressed protein confirmed by Dot Immuno Blot
Assay (DIBA). This expressed protein can be used for the production of antiserum. These aids in
the serological detection of Sweet potato leaf curl virus infection.
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