Transient Expression of Foreign Genes in Insect Cells (sf9) for Protein Functional Assay

Ju-Chun Chang; Se Jin Lee; Jae Su Kim; Chung-Hsiung Wang; Yu-Shin Nai

doi:10.3791/56693

A subscription to JoVE is required to view this content. Sign in or start your free trial.

Summary

This protocol describes a heat shock-induced protein expression system (pDHsp/V5-His/sf9 cell system), which can be used for either expressing foreign proteins or evaluating the anti-apoptotic activity of potential foreign proteins and their truncated amino acids in insect cells.

Abstract

The transient gene expression system is one of the most important technologies for performing protein functional analysis in the baculovirus in vitro cell culture system. This system was developed to express foreign genes under the control of the baculoviral promoter in transient expression plasmids. Furthermore, this system can be applied to a functional assay of either the baculovirus itself or foreign proteins. The most widely and commercially available transient gene expression system is developed based on the immediate-early gene (IE) promoter of Orgyia pseudotsugata multicapsid nucleopolyhedrovirus (OpMNPV). However, a low expression level of foreign genes in insect cells was observed. Therefore, a transient gene expression system was constructed for improving protein expression. In this system, recombinant plasmids were constructed to contain the target sequence under the control of the Drosophila heat shock 70 (Dhsp70) promoter. This protocol presents the application of this heat shock-based pDHsp/V5-His (V5 epitope with 6 histidine)/Spodoptera frugiperda cell (sf9 cell) system; this system is available not only for gene expression but also for evaluating the anti-apoptotic activity of candidate proteins in insect cells. Furthermore, this system can be either transfected with one recombinant plasmid or co-transfected two potentially functionally antagonistic recombinant plasmids in insect cells. The protocol demonstrates the efficiency of this system and provides a practical case of this technique.

Introduction

Two protein expression systems have been commonly used for producing proteins: prokaryote protein expression systems (Escherichia coli gene expression system) and eukaryote protein expression systems. One popular eukaryote protein expression system is the baculovirus expression vector system (BEVS)¹. Baculoviruses were first used as worldwide biological control agents of agricultural and forest pests. In the last few decades, baculoviruses were developed as biotechnological tools for protein expression vectors as well. The genomes of baculoviruses consist of double-stranded circular DNA and enveloped nucleocapsids². To date, more than seventy-eight baculovirus isolates have been sequenced³. Based on the temporal cascade of baculoviral gene expressions in host insect cells, the gene transcription could be classified into four temporal cascades, including immediate-early, delayed-early, late, and very late genes⁴.

BEVSs were designated so that the very late gene promoters (i.e., polyhedron or p10 promoter) were used to drive the target genes, while the recombinant baculovirus was generated by homologous recombination. Expression of foreign proteins in insect cells by recombinant baculovirus is similar to that of mammalian proteins in post-translational modifications (suited for glycoprotein production). Thus, the baculovirus has been widely used⁵^,⁶^,⁷. However, one limitation is the presence of different N-glycosylation pathways in insect cells⁷.

Therefore, a new baculovirus expression system, the transient gene expression system, was developed. This system expresses foreign genes under the drive of baculoviral immediate-early promoters (ie-1 promoter) in insect cells. By using this system, the target protein can be immediately expressed under the control of ie-1 promoter while modifying the N-glycosylation pathway in insect cells, resulting in better N-linked oligosaccharides⁷. Moreover, baculoviral immediate-early genes are transcribed by the host cell RNA polymerase II and do not require any viral factor for activation⁴. Therefore, foreign proteins can be expressed in insect cells within a short time. To date, the transient gene expression system is one of the most important technologies for performing protein functional assays in the baculovirus in vitro cell culture system. The system can be applied to analyze the function of either baculovirus or foreign proteins. One of the commercially available transient gene expression systems is based on the immediate-early gene (IE) promoters of Orgyia pseudotsugata multicapsid nucleopolyhedrovirus (OpMNPV) (OpIE2 and OpIE1 promoters).

However, the lower expression level of foreign genes in insect cells was still a problem when the OpIE promoter-based transient gene expression system was used⁸^,⁹^,¹⁰. Thus, another transient gene expression system was constructed based on the promoter of the Drosophila heat shock protein 70 (hsp70) gene⁸^,⁹. The promoter of hsp70 works more efficiently than baculoviral IE promoter when induced by heat shock in insect cells¹⁰. In this system, the target genes were expressed under the drive of Drosophila heat shock 70 (Dhsp70) promoter. Foreign genes can be easily cloned into the transient gene expression plasmid by PCR-based cloning methods. Furthermore, the control of timing for gene expression can be performed by heat shock induction.

In this report, we follow the approach and express three different truncations of the baculoviral gene (inhibitor of apoptosis 3, iap3 from Lymantria xylina MNPV) by using the heat shock-based transient protein expression system and further apply these expressed proteins on anti-apoptotic activity analysis. This system can either express foreign proteins quickly or be further applied to the evaluation of protein anti-apoptotic activity in sf9 cells, while also having the potential to be applied to other protein activity assays.

Protocol

1. Preparations

Insect cell culture
1. Prepare 50 mL of cell culture medium. To do so, add 500 µL of antibiotics (Amphotericin B = 0.25 µg/mL, Penicillin = 100 unit/mL, Streptomycin = 100 µg/mL) and 5 mL of heat-inactivated fetal bovine serum in serum-free cell culture medium (without FBS or antibiotics).
  NOTE: Heat the fetal bovine serum at 65 °C for 30 min in a water bath before use.
2. Maintain Spodoptera frugiperda (Lepidoptera: Noctuidae), sf9 insect cells. Detach ca. 80% of the cells from 25 cm² cell culture flask by shaking the flask and check under light microscopy. Then, transfer 50% of the cell suspension to a new 25 cm² cell culture flask and allow the cells to attach for 15 min at room temperature. Replace the medium with 5 mL fresh cell culture medium and grow in an incubator at 28 °C. Passage cells every 2 to 3 days depending on the cell growth.
Preparation of plasmids for cell transfection
1. Insert the target DNA fragments (e.g., Lymantria xylina MNPV (LyxyMNPV) iap3 gene and its deletion constructs) into pDHsp/V5-His by PCR-based cloning method¹¹. Check the growth of transformed colonies by colony PCR using PCR Master Mix (2X) and the pDhsp-F2/Op-IE2R primer set. Confirm the plasmid sequences by commercial sequencing service.
  NOTE: Table 1 lists the primers used for PCR and the corresponding constructs.
2. Culture single sequenced bacterial colonies, which contain the aforementioned plasmid constructions (step 1.2) in 200 mL LB medium containing selected antibiotics (50 µg/mL), respectively.
3. Extract the plasmids from the cultured E. coli using Midi Plasmid Kit according to manufacturer's instructions¹².
Prepare plating medium by mixing 1.5 mL of cell culture medium and 8.5 mL of serum-free cell culture medium.
Prepare Actinomycin D (ActD) cell culture medium by adding 1.5 µL of ActD stock (1 mg/mL) into 10 mL of cell culture medium (final concentration = 150 ng/mL). Store at 4 °C.

2. Protein transient expression

Cell seeding
1. Harvest the sf9 cells by shaking culture flask, topple and fall the cell suspension to 50 mL tube, and transfer 10 µL to hemocytometer by a P10 pipette. Count the cell number under a light microscope.
2. Plate 3 × 10⁵sf9 cells into each well in a 24-well plate for 15 min at room temperature. Replace the medium with 0.5 mL of plating medium.
Transfection of plasmids
1. Dilute cell transfection reagent: Dilute 8 µL of cell transfection reagent in 100 µL serum-free cell culture medium and mix by vortexing for 1 s.
2. Add 2 µg of plasmid DNA (pDHsp70-Ac-P35/V5-His or pDHsp70-Ly-IAP3/V5-His or pDHsp70-Ly-IAP3-BIR/V5-His or pDHsp70-Ly-IAP3-RING/V5-His) into 100 µL of serum-free cell culture medium and mix by vortexing for 1 s (Figure 2).
3. Combine the diluted plasmid DNA and diluted cell transfection reagent (210 µL), and mix by vortexing for 1 s. Incubate for 30 min at room temperature.
4. Add 210 µL of DNA transfection reagent mixture dropwise onto the cells by a P1000 pipette. Incubate at 28 °C for 5 h.
5. Replace the plating medium with 0.5 mL of cell culture medium using a P1000 pipette. Seal the 24-well plate with tape and incubate the cells at 28 °C for 16 h.
Heat shock the transfected cells: Put the plate in a 42 °C water bath (floating on the water surface). Heat for 30 min and return the 24-well plate to the 28 °C incubator.
Detection of protein expression
1. After 1 h or 5 h heat shock,wash the cells with 0.5 mL of 1x PBS buffer briefly three times.
  NOTE: Dilute 10x PBS buffer to 1x PBS buffer by adding 1 mL of 10x PBS buffer to 9 mL sterilized ddH₂O
2. Lyse the cells with 40 µL of 1x SDS Loading Dye by pipetting up and down.
  NOTE: Dilute 4x SDS Loading Dye by mixing 30 µL of 1x PBS buffer and 10 µL of 4x SDS Sample Buffer.
3. Heat the protein samples at 98 °C for 10 min in a heat block, spin down for 1 min, and put on ice for Western blot assay.
4. Western blot assay
  Follow the procedure of Western blot assay from Eslami and Lujan¹³. Run SDS-PAGE gels¹⁴: one gel subjected to Coomassie blue staining (loading control for checking that the quantity of protein samples loaded in each well is equal in amount) and the other subjected to Western blot assay, according to Eslami and Lujan¹³.
5. Detect V5-tagged fusion proteins with rabbit anti-V5 antibody (5 mg/mL) (1:5000 dilution in TBST buffer to working concentration 1 µg/mL) and goat anti-rabbit IgG-horseradish peroxidase (HRP) conjugate (0.8 mg/mL) (1:10000 dilution in TBST buffer to working concentration 0.08 µg/mL).
  NOTE: Adjust the percentage of polyacrylamide to 17.5% when the protein molecular weight to be <17 kDa.

3. Anti-apoptotic activity assay

Gene-induced cell apoptosis: Repeat the aforementioned procedure from 2.1 to 2.3. Co-transfect 1 µg of pDHsp/D-rpr/FLAG-His plasmid DNA (containing apoptosis inducer gene) with 1 µg of plasmid DNA [pDHsp70/V5-His vector (negative control), pDHsp70-Ac-P35/V5-His (positive control), pDHsp70-Ly-IAP3/V5-His, pDHsp70-Ly-IAP3-BIR/V5-His or pDHsp70-Ly-IAP3-RING/V5-His, respectively.]. At 5 h post-heat shock treatment, conduct the cell viability assay (Figure 2).
Chemical-induced cell apoptosis: Repeat the aforementioned procedure from 2.1 to 2.3. In step 2.1.2, plate 1 x 10⁶sf9 cells into each well in a 6-well plate. Transfect 4 µg of plasmid DNA [pDHsp70/V5-His vector (negative control), pDHsp70-Ac-P35/V5-His (positive control), pDHsp70-Ly-IAP3/V5-His, pDHsp70-Ly-IAP3-BIR/V5-His or pDHsp70-Ly-IAP3-RING/V5-His, respectively.]. At 5 h post-heat shock, treat sf9 cells with 2mL of ActD cell culture medium for 16 h and conduct the cell viability assay (Figure 2).
NOTE: Minimum volume to cover one well of 6-well plate is 1 mL.
Perform the above anti-apoptotic activity assay experiments, including 3.1 and 3.2 in triplicates.

4. Cell viability assay

Wash the treated cells by adding 1 mL of 1x PBS buffer for 1 min 3 times. Resuspend the cells by pipetting 1 mL 1x PBS buffer containing 0.04% trypan blue and stain for 3 min at room temperature. Transfer the cell suspension into a 1.5 mL microtube.
NOTE: Dilute 0.4% trypan blue solution by mixing 9 mL of 1x PBS buffer and 1 mL 0.4% trypan blue solution.
Transfer 10 µL trypan blue-stained cell suspension to the hemocytometer with a P10 pipette and count the viable intact cells under a light microscope.
Statistical analysis
1. Calculate the recorded data and present as the means ± S.D. for all counts.
2. Analyze the data using the Student's two-tailed t-test by with Microsoft Excel. Define statistically significant data as P-value <0.05.

Results

The full length and other two truncations (BIR and RING domains) of Ly-IAP3 from LyxyMNPV were overexpressed in sf9 cells, based on the heat shock-based pDHsp/V5-His/Spodoptera frugiperda cell (sf9 cell) system. The pDHsp/V5-His contained a Drosophila heat shock protein promoter, which drives downstream gene expression at a temperature of 42 °C condition by using cellular transcriptional factors and the translation system (Figure 1)

Discussion

The concept of heat shock-based pDHsp/V5-His/sf9 cell system was first described by Clem et al. in 1994⁸. Comparison of the baculoviral gene promoter (IE1) and Drosophila hsp70 showed that hsp70 had a higher efficiency in mosquito cells¹⁰. Furthermore, due to the heat shock induction, the timing of protein expression could be controlled precisely after heat shock treatment. This system was then applied for protein functional assays of shr...

Disclosures

The authors declare that they have no competing financial interests.

Acknowledgements

We thank Dr. Jian-Horng Leu of Institute of Marine Biology, National Taiwan Ocean University for providing 3 plasmid constructions. This research was supported by Grant 106-2311-B-197 -001 - from the Ministry of Science and Technology (MOST).

Materials

Name	Company	Catalog Number	Comments
Antibiotic-Antimycotic, 100X	Gibco	15240-062	for insect cell culture
Certified Foetal Bovine Serum	Bioind	04-001-1A
Sf-900 II SFM	Thermo Fisher	10902096	serum-free cell culture medium
Sf9 cells	ATCC	CRL-1711
25cm2 cell culture flask	Nunc, Thermo Fisher	156340
Inverted light microscopy	WHITED	WHITED WI-400
RBC HIT Competent Cell	Bioman	RH618-J80	Escherichia coli (DH5α)
L.B. Broth (Miller)	Bioman	LBL407
Agar, Bacteriological Grade	Bioman	AGR001
Zeocin	Invitrogen	ant-zn-1	selection antibiotic
PCR Master Mix (2X)	ThermoFisher	K0171
Geneaid Midi Plasmid Kit (Endotoxin Free)	Geneaid	PIE25
Actinomycin D	SIGMA	A9415
Corning 50 mL centrifuge tubes	SIGMA	CLS430829-500EA	50 mL tubes
Hemocytometer	Gizmo Supply Co	B-CNT-SLDE-V2
24-Well Multidish	Nunc, Thermo Fisher	142475	24-well plate
Cellfectin II Reagent	Thermo Fisher	10362100	cell transfectin reagent
PBS-Phosphate-Buffered Saline (10X) pH 7.4	Thermo Fisher	AM9624
4×SDS Loading Dye	Bioman	P1001
Immobilon-P (PVDF Blotting Membranes)	Merck Milipore	IPVH00010	PVDF membranes
Mini Trans-Blot Cell system	BIO-RED	1703930	Blotting device
Ponceau S solution	SIGMA	6226-79-5
Anti-V5	SIGMA	V8137	rabbit anti-V5 antibody
Goat anti-rabbit IgG-horseradish peroxidase (HRP)	Jackson	111-035-003
Tween 20	Merck	817072
6-Well Multidish	Nunc, Thermo Fisher	145380
0.4 % trypan blue solution	AMRESCO	K940-100ML
P10 pipetman	Gilson	F144802
P1000 pipetman	Gilson	F123602
Tape	Symbio	PPS7	24 well tape ( 19 mm×36 M)

References

Miller, L. K. Baculoviruses as gene expression vectors. Annual Reviews in Microbiology. 42 (1), 177-199 (1988).
Theilmann, D. A., Fauquet, C. M., Mayo, M. A., Maniloff, J., Desselberger, U., Ball, L. A., et al. Family Baculoviridae. Virus Taxonomy: Eighth Report of the International Committee on Taxonomy of Viruses. , 1129-1185 (2005).
Nai, Y. S., Huang, Y. F., Chen, T. H., Chiu, K. P., Wang, C. H., Shields, V. D. C. Determination of nucleopolyhedrovirus' taxonomic position. Biological Control of Pest and Vector Insects. , 169-200 (2017).
Friesen, P. D., Miller, L. K. Regulation of baculovirus early gene expression. The Baculoviruses. , 141-170 (1997).
Smith, G. E., Summers, M., Fraser, M. Production of human beta interferon in insect cells infected with a baculovirus expression vector. Mol. Cell. Biol. 3 (12), 2156-2165 (1983).
Luckow, V. A., Summers, M. D. Trends in the development of baculovirus expression vectors. Nature Biotechnol. 6 (1), 47-55 (1988).
Jarvis, D. L., Finn, E. E. Modifying the insect cell N-glycosylation pathway with immediate early baculovirus expression vectors. Nature Biotechnol. 14 (1996), 1288-1292 (1996).
Clem, R. J., Miller, L. K. Control of programmed cell death by the baculovirus genes p35 and iap. Mol. Cell. Biol. 14, 5212-5222 (1994).
Leu, J. H., Kuo, Y. C., Kou, G. H., Lo, C. F. Molecular cloning and characterization of an inhibitor of apoptosis protein (IAP) from the tiger shrimp, Penaeus monodon. Dev. Comp. Immunol. 32, 121-133 (2008).
Zhao, Y. G., Eggleston, P. E. Comparative analysis of promoters for transient gene expression in cultured mosquito cells. Insect Mol. Biol. 8 (1), 31-38 (1999).
Nai, Y. S., Yang, Y. T., Kim, J. S., Wu, C. Y., Chen, Y. W., Wang, C. H. Baculoviral IAP2 and IAP3 encoded by Lymantria xylina multiple nucleopolyhedrovirus (LyxyMNPV) suppress insect cell apoptosis in a transient expression assay. Appl. Entomol. Zool. 51, 305-316 (2016).
Eslami, A., Lujan, J. Western Blotting: Sample Preparation to Detection. J. Vis. Exp. (44), e2359 (2010).
. Basic Methods in Cellular and Molecular Biology. Separating Protein with SDS-PAGE Available from: https://www.jove.com/science-education/5058/separating-protein-with-sds-page (2017)
Vucic, D., Kaiser, W. J., Harvey, A. J., Miller, L. K. Inhibition of reaper-induced apoptosis by interaction with inhibitor of apoptosis proteins (IAPs). Proc. Natl. Acad. Sci. USA. 94, 10183-10188 (1997).

Reprints and Permissions

Request permission to reuse the text or figures of this JoVE article

Request Permission

Explore More Articles

Transient Gene Expression Insect Cells Sf9 Protein Functional Assay Anti apoptotic Activity Heat Shock Induction Protein Expression Cell Culture Transfection IAP3

This article has been published

Video Coming Soon

Keep me updated: