Abstract
Low temperature induces diapause in locusts. However, the physiological processes and initiation mechanism of diapause are not well understood. To understand the molecular basis of diapause, ‘omics’ analyses were performed to examine the differences between diapause and non-diapause eggs at both transcriptional and translational levels. Results indicated that a total of 62,241 mRNAs and 212 proteins were differentially expressed. Among them, 116 transcripts had concurrent transcription and translation profiles. Up-regulated genes related to diapause included glutathiones-S-transferase et al. and down-regulated genes including juvenile hormone esterase-like protein et al. KEGG analysis mapped 7,243 and 99 differentially expressed genes and proteins, to 83 and 25 pathways, respectively. Correlation enriched pathways indicated that there were nine identical pathways related to diapause. Gene Ontology analysis placed these genes and proteins into three categories and a higher proportion of genes related to metabolism was up-regulated than down-regulated. Furthermore, three up-regulated pathways were linked to cryoprotection. This study demonstrates the applicability of high-throughput omics tools to identify molecules linked to diapause in the locust. In addition, it reveals cellular metabolism in diapause eggs is more active than in non-diapause eggs and up-regulated enzymes may play roles in cryoprotection and storing energy for diapause and post-diapause stages.
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Introduction
Diapause is an adaptation to seasonality that is widespread across invertebrate taxa1,2. There are two forms of insect diapause: facultative diapause, which is a response to key stimuli from the environment, andobligatory diapause, which is a fixed component of ontogeny1. The migratory locust is an embryonic diapause insect of the facultative diapause type3,4. These pests can move and settle in new habitats, which may be a fixed behavioral strategy that results from long-term evolutionary adaptation5. Diapause may serve to adapt the migratory locust to factors such as temperature, photoperiod and latitude6,7. For example, the diapause rate of the migratory locust in high latitude locations is higher than that observed in low latitude locations8 and short photoperiod and low temperatures are known to increase the number of locusts entering diapause6,7,9. More importantly, incubation temperature influences the diapause rate of locust eggs; the proportion of embryo reversal is strengthened upon temperature increase10,11. In addition, we identified an interesting phenomenon in Tianjin, a location that has supported two generations of migratory locusts, locusta migratoria L., according to historical records. Most hatchlings of the 3rd generation emerged in autumn due to the overwintering of eggs, but this phenomenon decreased dramatically after A.D. 199912,13 and may have been linked to temperature variation during autumn, as high temperatures have been shown to promote egg development and to result in the emergence of 3rd-generation hatchlings. However, the influence of temperature on locust diapause is unknown.
Locust eggs are extremely sensitive to temperature before anatrepsis, which leads parts of the embryo to hatch upon exposure to high temperatures during this period6,7,14. When degree-day (DD) was higher than 150 heat units prior to anatrepsis, all of the eggs transformed into hatchlings. When DD was only 66 heat units, 64.3% of embryos entered diapause11. In this study, we reared locusts at high and low temperatures until adults oviposited, then overwintered eggs were collected when DD reached 50 heat units9,11. Thus, diapause eggs were exposed to low temperatures and non-diapause eggs were maintained at high temperatures. We compared diapause and non-diapause eggs at the transcriptome (RNA-seq) and proteome (iTRAQ) levels15,16 to enhance our understanding of the genetic and molecular mechanisms underlying diapause in an agriculturally important insect pest.
Results
Omics analyses
Diapause and non-diapause locust egg transcriptomes were sequenced individually, which generated approximately 135–138 million clean reads, 12.2–12.4 billion nucleotides, 210–223 thousand contigs and 94–118 thousand unigenes for each library (Table 1). To uncover the molecular events underlying these transcriptomic profiles, we aligned unigene sequences to protein databases, including NR, Swiss-Prot, KEGG and COG (e-value < 0.00001) by blastx and nucleotide database NT (e-value < 0.00001) by blastn, retrieving proteins with the highest sequence similarity to the given unigenes along with their functional annotations. Of the 100,490 unigenes, we found that 36,765 were annotated.
The total number of sequences identified by mass spectrometry of locust egg proteomes was 271,268, which represented 2,787 peptide spectra and 2,634 distinct peptides (Table 2). Of the 2,634 peptides identified, more than 40% (1,078) were assigned to a putative protein by homology search against the non-redundant (NR) database, leaving approximately 60% (1,556) of the peptides unidentified. Among these annotated proteins, 447 were hypothetical, putative, or predicted.
Differentially expressed genes (DEGs) between diapause and non-diapause locust eggs
Following temperature treatment, a total of 37,516 and 24,725 up- and down-regulated transcripts, respectively, were differentially expressed (FDR ≤ 0.001 and |log2Ratio ≥ 1) between diapause and non-diapause locust eggs (Fig. 1A). Most of these transcripts (15,896 and 16054, 66%), however, were expressed within a 2- to 10-fold difference (Fig. 2).
Table S1 shows the GO classification of 62,241 transcripts that were differentially expressed between diapause and non-diapause locust eggs (≥2-fold change, FDR ≤ 0.001). With Blast2GO, 9,696 differentially expressed transcripts were assigned to 56 GO classes (Fig. 3A). The majority of these genes were assigned to categories such as biological process, cellular component, molecular function, response to biological regulation, cellular process, metabolic process, single-organism process, binding, catalytic activity, organelle part, cell and cell part (Table S1). In the up-regulated group, most genes were assigned to the mucin, heat shock protein, ATP-binding cassette, transcription initiation factor and DNA-directed RNA polymerase categories. To investigate their biological functions, 10,351 differentially expressed genes were mapped to 259 pathways in the KEGG database. To investigate which biological pathways were active when exposed to diapause treatment, 7,243 differently expressed genes were assigned to reference pathways in KEGG. As a result, 83 pathways were substantially enriched (p-value < 0.05), including “Metabolic Pathway” and “Ribosome” (Table 3). Specifically, 154 genes encoding enzymes involved in starch and sucrose metabolism pathways were highly enriched, including trehalose, 6-phosphate phosphatase, trehalase, glucokinase and starch phosphorylase (Table S2). Interestingly, we also found that 2,459 up-regulated and 365 down-regulated genes were linked to metabolic pathways (Table S3). The up-regulated transcripts included glutathiones-S-transferase (GST), UDP-glucuronosyl transferase (UGT), transforming growth factor-β-receptor (TGF), insulin-like growth factor receptor (IGF), nuclear receptor, fork head transcription factor (FOXO), transient receptor potential cation channel subfamily A member 1(TRPA1), inositol-3-phosphate synthase (PIP3), acetyl-Coenzyme A acyltransferase (ACAA), catalase, glucose dehydrogenase, heat shock proteins (HSPs), glycerol kinase and the cytochrome c oxidase, cytochrome p450 (Table S2, S3). The down-regulated genes included juvenile hormone esterase-like protein, hemocyanin subunit, hexamerin-like protein and NADH-dehydrogenase (Table S2, S3).
Temperature-dependent protein expression in diapause and non-diapause locust eggs
After temperature challenge, 212 differentially expressed proteins (p-value ≤ 0.05) were identified between diapause and non-diapause locust eggs. Among them, 65 proteins were up-regulated (≥1.2-fold, p-value ≤ 0.05) and 147 were down-regulated (≤0.8-fold, p-value ≤ 0.05) (Fig. 1B). Following in-gel digestion by trypsin, the peptides were identified by liquid chromatography-electrospray ionization multi stage mass spectrometry (LC-ESI-MS/MS; Table S4). Cu/Zn superoxide dismutase and peroxiredoxin-1, which are found in the peroxisome, were up-regulated by 3.233- and 1.393-fold, respectively, in diapause eggs relative to non-diapause eggs17. Other up-regulated peptides in diapause eggs included juvenile hormone esterase (11.211-fold), which demethylates the insect juvenile hormones JH (1) and JH (3) but does not hydrolyze the analogous ethyl or isopropyl esters18; (1,3)-β-glucan synthase (2.801-fold), which plays an important role in catalyzing the transfer of sugar moieties from activated donor molecules to specific acceptor molecules to form glycosidic bonds19; eukaryotic translation initiation factor 4A (1.936- fold), which is associated with protein translation initiation and elongation20; and lipase (1.795-fold), which performs essential roles in the digestion, transport and processing of dietary lipids21. In addition, proteins related to energy regulation, protein transport and metabolism were differentially expressed between diapause and non-diapause locust eggs (Table S5). Peptides that were down-regulated in the diapause eggs included hemocyanin subunit type 2 (−7.143-fold), which is involved in energy storage, osmotic pressure maintenance and molt regulation22; fatty acid-binding protein (−4.255-fold), which may play an important role in up-regulating heat shock proteins during diapause23; phenoloxidase subunit 1 (−3.300-fold), which performs essential roles in the synthesis of hemocyanin C, M, N and tyrosinase24; and alcohol dehydrogenase class-3-like (−1.212-fold),which is associated with aromatic compound and fatty acid degradation, glycolysis, gluconeogenesis and tyrosine, retinol and xenobiotic metabolism25.
To correlate protein and mRNA expression profiles, accession numbers from the proteomic dataset were extracted and compared with the annotated RNA-seq libraries. Correlation between the differentially expressed proteins and genes showed that there were only 116 genes/proteins related to diapause (Fig. 4). Tables S6 and S7 show the correlation between mRNA and protein and the correlation coefficients between the protein and gene expression profiles were 0.8078 and −0.5775 (Fig. 5, Table S6, S7).
Gene ontology and pathway analysis
Among the 212 differentially expressed proteins, 156 were subcategorized into 44 hierarchically structured GO classes, including 22 Biological Process, 13 Cellular Component and 9 Molecular Function (Fig. 3B) categories. Specifically, “cellular process” (104, 66.7%), “metabolic process” (104, 66.7%) and “single-organism process” (71, 45.5%) were highly represented in “Biological Process”, whereas “cell” (95, 60.9%), “cell part” (95, 60.9%) and “organelle” (73, 46.8%) were the most common categories in “Cellular Component”. In “Molecular Function”, the top three categories were “catalytic activity” (98, 62.8%), “binding” (87, 55.8%) and “structural molecule activity” (21, 13.5%) (Fig. 3B, Table S6). Ninety-nine differentially expressed proteins were allocated to the reference pathways in KEGG (Table 4). As a result, 25 pathways were enriched (p-value ≤ 0.05, Table 4). Correlation of the enriched pathways for differentially expressed genes and proteins showed that there were 9 identical pathways related to diapause, including those mediating, peroxisome, glyoxylate and dicarboxylate metabolism, melanogenesis, tyrosine metabolism, riboflavin metabolism, retinol metabolism, pentose and glucuronate interconversion and glutathione metabolism (Tables 3,4).
We investigated which biological pathways were active following diapause treatment and found that 3 pathways played an important role, including (i) Starch and sucrose metabolism (KEGG: Map00500), which involved α, α’-D-Trehalose synthesis from glycogen and included the up-regulation of maltase-glucoamylase, glycogen debranching enzyme, hexokinase, starch phosphorylase, glycogen synthase, glucose-6-phosphate isomerase, phosphoglucomutase, UTP-glucose-1-phosphate uridylyltransferase, trehalose 6-phosphate synthase and trehalose 6-phosphate phosphatase; (ii) Glycolysis and gluconeogenesis (KEGG: Map00010); and (iii) Glycerolipid metabolism (KEGG: Map00561), which involves glycerol synthesis from glucose and the up-regulation of aldose-1-epimerase, hexokinase, glucokinase, ADP-dependent glucokinase, phosphoglucomutase, glucose-6-phosphate 1-epimerase, glucose-6-phosphate isomerase, 6-phosphofructokinase, triosephosphate isomerase, glycerate kinase, aldehyde dehydrogenase, alcohol dehydrogenase and aldehyde reductase during the pre-diapause stage. These up-regulated enzymes enabled diapause eggs to synthesize cryoprotectants (e.g., trehalose and glycerinum) and to store energy for diapause and post-diapause stages.
Discussion
Insect diapause can be divided into the pre-diapause, diapause and post-diapause stages26 and insects in the pre-diapause stage are able to synthesize cryoprotectants and store energy for later developmental stages27,28. However, the definition and naming of the pre-diapause stage are unsettled and occasionally ambiguous in the literature, particularly for Locusta migratoria L9. The induction factors in obligative diapause insects and facultative diapause insects (e.g., L. migratoria) were analyzed and a comparison of the results suggested that the entrance of the latter to diapause was determined by the photoperiod and incubation temperature29. It is a fixed component of ontogeny, e.g., Sarcophaga crassipalpis is pupal diapause30, whereas Drosophila montana is adult reproductive diapause31. Overall, 100% of them entered diapause and remained in the stage until stimuli triggered further development in the spring1. However, for L. migratoria, photoperiod only influenced the development of ovary7, which was not the most important factor influencing the diapause rate of locust eggs. Therefore temperature plays a determinative role and the effects of temperature can be subdivided as follows: first, low temperature influenced the development of adults;for example, if the temperature was lower than 21 °C32, females could not support the reproductive process and the fertilization process in adults may be affected9. Second, incubation temperature influenced the development of eggs during the anatrepsis stage11. Hence, we speculated that the pre-diapause stage of L. migratoria began at the point of female fertilization and ended at embryo anatrepsis. This theory could explain why only parts of eggs would enter diapause and why the diapause rate varied from northern to southern China, as incubation temperature differed during the processes of fertilization and embryo anatrepsis8,11. Thus, overwintered eggs treated at 50 DD, which coincided with the pre-diapause stage of the migratory locust, were collected and prepared for omics analyses.
Transcriptome sequencing indicated that physiological metabolism had been activated and up-regulated transcripts (37,516) were more abundant than down-regulated transcripts (24,725) (Fig. 2). These results can be used to study the mechanisms underlying diapause in L. migratoria33. A correlation analysis of differentially expressed proteins and genes showed that a subset ofgenes and proteins were expressed with the same trend during the pre-diapause stage (Fig. 5, Tables S6, S7). Genes including glutathiones-S-transferase, UDP-glucuronosyl transferase and transforming growth factor-β-receptor were up-regulated, whereas hemocyanin subunit, hexamerin-like protein and NADH dehydrogenase were among the genes down-regulated at both the transcriptional and translational levels (Table S2, S3). Physiologically similar phenotypes were identified in Sarcophag acrassipalpis, Drosophila melanogaster and Caenorhabditis elegans transcriptomes34. However, we found that some genes, including juvenile hormone esterase-like protein, were up-regulated at the translational level but down-regulated at the transcriptional level. This effect can be attributed to differences in expression time34. Changes in KEGG pathways and enzymes suggest that all enzymes in the three pathways related to cryoprotection were up-regulated, in contrast to the data obtained from Bombyx mori, although the silkworm utilizes the same cryoprotectants28. For example, sorbitol dehydrogenase expression was inhibited and glycogen phosphorylase A was enhanced for B. mori. However, we did not detect sorbitol dehydrogenase gene expression in locust eggs35,36. Diapause eggs produced trehalose and glycerinum, as supported by data from Li et al.37, but we detected no sorbitol dehydrogenase38,39. These differences may be due to differences in geographical sampling and diapause stage40,41.
Insect diapause-related endocrine regulation includes diapause hormone and insulin pathways. For example, diapause hormone and G-couple receptor in the ovary combine to synthesize cryoprotectants in B. mori28,42,43,44 and the insulin signaling system promotes Drosophila melanogaster diapause via FOXO phosphorylation in the PI3K/Akt pathway45, whereas juvenile hormone synthesis promoted Culex pipiens diapause46. We discovered that insulin growth factor and insulin receptor were up-regulated in the migratory locust, which enhances the proportion of juvenile hormone. This may pertain to diapause47, but not via the same mechanism as in the mosquito, Culex pipiens45,48. Studies have reported that many temperature-related genes, including fork head transcription factor, heat shock protein and transient receptor potential cation channel subfamily A member 1 might play a role in insect diapause metabolism46,49,50. We found that these genes were up-regulated (Figs 2,3), but how they affect migratory locust diapause is unknown. Additionally, genes and proteins expressed during the diapause and post-diapause stages require further study to understand the mechanism of locust diapause.
Materials & Methods
Ethics statement
The migratory locust, Locusta migratoria L. strains used in this study were initially collected in the field at Tianjin in 2007 and have since been maintained in a greenhouse at the Institute of Plant Protection, Chinese Academy of Agricultural Sciences. Species of the genus Acridoidea are common agricultural pests and are not included in the “List of Protected Animals in China”. No specific permits were required for the described field studies.
Temperature treatment
To obtain diapause and non-diapause eggs, we raised the oriental migratory locust in growth cabinets (PRX-350B-30) under low and high temperature regimes6. We recorded the daily temperature at Tianjian, from 16 July to 6 November 2012, as a reference (reference value), then used two different cabinets to mimic natural the natural daily temperature cycles of (reference value+1) for the high temperature regime and (reference value-1) for low temperature regime11. The photoperiod regime used in the experiment was L:D = 12:12 and the relative humidity (RH) was kept at ~60% for eggs and ~80% for nymph and adults. We recorded 24-h temperature data on each day for each growth cabinet using a HOBO Pro v2 logger and the results showed that the DD of the high temperature regime was 840 heat units and that DD of the low temperature regime was 678 heat units32.
Sample preparation
More than 2,000 locust eggs were collected from the same generation, divided into two groups and reared in the two growth cabinets for a whole generation11. After adults oviposited, we recorded the hatchlings on each day in each of the two growth cabinets. We found that the diapause rate of overwintering eggs at the low temperature regime was 64.3% (diapause eggs, only 35.7% hatchlings emergence in the growth cabinet), whereas all eggs hatched at the high temperature regime (non-diapause eggs, 100% hatchling emergence in the growth cabinet)11. Diapause and non-diapause eggs were collected when DD reached 50 heat units9,11 and were immediately snap-frozen in liquid nitrogen and stored at −80 °C.
RNA-seq library preparation and sequencing
Total RNA was isolated from diapause and non-diapause locust egg samples, respectively, with Trizol (Invitrogen) according to the manufacturer’s protocol. The quantity and quality of RNA were determined with a Nanodrop ND-1000. To remove residual DNA contamination, total RNA was treated with RNase-free DNase I (New England BioLabs). mRNA was purified from 6 μg of total RNA from each sample with Dynaloligo (dT) beads (Invitrogen) and was then fragmented using an RNA fragmentation kit (Ambion). The first cDNA strand was synthesized using random hexamer primers. The double-stranded cDNA fragments were processed by end repair using T4 DNA polymerase, Klenow DNA polymerase and T4 polynucleotide kinase (NEB), followed by a single adenine base addition using Klenow 39 to 59 exo-polymerase and was concluded by ligation with Illumina’s adaptor. The products were purified using a QiaQuick PCR extraction kit (QiaGen) and enriched by PCR amplification. Finally, the library products were subjected to sequencing analysis on the Illumina HiSeqTM 2500 platform.
Annotation and de novo gene expression
Raw reads were transformed into clean reads by removing the adaptor sequences, reads with unknown nucleotides larger than 5%, empty sequences (sequences with an adaptor but no reads) and low-quality sequences (the rate of reads for which quality value ≤ 10 is more than 20%)51. Transcriptome de novo assembly was carried out with the Trinity short read assembly program. Trinity combines three independent software modules: Inchworm, Chrysalis and Butterfly, which are applied sequentially to process large volumes of RNA-seq reads52. Trinity partitions the sequence data into many individual de Bruijn graphs, each representing the transcriptional complexity at a given gene or locus and then processes each graph independently to extract full-length splicing isoforms and to tease apart transcripts derived from paralogous genes. The calculation of Unigene expression uses the FPKM (RPKM) method (Fragments Per kb per Million reads)53. The formulas for computing FPKM and RPKM are the same. The only difference between them is the method used to compute the parameters of N and C. If both pairs of reads were aligned to a gene, we treated them as 1 fragment with FPKM but as two reads with RPKM. Both algorithms are rational. For functional annotation, distinct sequences were searched via BLAST against the NCBI NR database with a cut-off E-value of 10−5. In addition, Blast2GO (http://www.blast2go.org) was used to assign Gene Ontology terms (http://www.geneontology.org), while the Kyoto Encyclopedia of Genes and Genomes (KEGG, http://www.genome.jp/kegg/ or http://www.kegg.jp/), a database resource that integrates genomic, chemical and systemic functional information, was adopted to annotate molecular networks (pathways).
Screening for differentially expressed genes
Referring to “The significance of digital gene expression profiles”, which has been cited hundreds of times54, we developed a rigorous algorithm to identify differentially expressed genes between two samples. The null hypothesis and alternative hypothesis to identify differentially expressed genes are defined as follows:
H0:a gene has the same expression level in two samples
H1:a gene has different expression levels in two samples
We denote x as the number of fragments that uniquely map to gene A. For each transcript representing a small fraction of the library, p(x) follows the Poisson distribution closely.
The total fragment number of sample 1 is N1 and the total fragment number of sample 2 is N2; gene A comprises x fragments in sample 1 and y fragments in sample 2. The probability of gene A being expressed equally between two samples can be calculated using the following formula:
Or
Here
When we perform thousands of hypothesis tests, a suitable P-value for an individual test is not sufficient to guarantee a low rate of false discovery; thus, we must perform a multiple testing correction for each individual hypothesis test to guarantee a low false discovery rate overall. FDR (False Discovery Rate) control is a statistical method used in multiple hypothesis testing to correct for p-value. In practical terms, the FDR is the expected false discovery rate; for example, if 1000 observations were experimentally predicted to differ and the maximum FDR for these observations was 0.1, then 100 of these observations would be expected to be false discoveries (refer to Benjamini (2001) for details). When we have an FDR, we use the ratio of FPKMs of the two samples concurrently. The smaller the FDR is and the larger the ratio is, the larger the difference of the expression level between the two samples will be. In our analysis, we chose those samples with FDR ≤ 0.001 and a ratio larger than 2 DEGs and then carried out GO functional analysis and KEGG Pathway analysis55.
Protein quantification and database search using iTRAQ labeling
Locust egg samples were dissected in lysis buffer (7 M urea, 2 Mthiourea, 4% CHAPS, 40 mMTris-HCl, pH 8.5) and 1 mM PMSF (phenyl methane sulfonyl fluoride) and 2 mM EDTA (ethylene diamine tetraacetic acid) were added after dissection. After 5 min, 10 mM DTT was added to the lysis solution, which was then centrifuged at 4 °C, 30,000 × g for 15 min. The supernatant was collected and the concentration of total proteins was determined using a 2DQuantification Kit (GE Healthcare)56. For quality check, 30 mg of total protein from each sample was subjected to SDS-PAGE analysis. After, 100 ml protein from each sample was digested with trypsin gold (Promega) (protein: trypsin = 30:1) at 37 °C for 16 h and the resultant peptides were dried by vacuum centrifugation. The peptides were reconstituted in 0.5 M TEAB and processed according to the manufacturer’s protocol for 8-plex iTRAQ (Applied Biosystems, Inc)57. Samples (100 mg total protein/sample) from non-diapause and diapause locust eggs were labeled with iTRAQ tags 115 and 119, respectively. Then, pooled mixtures of iTRAQ-labeled peptides were fractionated by SCX chromatography (Phenomenex, Inc, USA) using a Shimadzu LC-20AB HPLC Pump system. Collected fractions were pooled into 10 final fractions and analyzed by nano LC-MS/MS analysis after desalting by Strata XC18 column (Phenomenex) and vacuum dried. Nano LC-MS/MS analysis of each of these fractions was performed using a LTQ-OrbitrapVelos mass spectrometer (Thermo Fisher Scientific Inc. Rockford, IL, USA) equipped with nano electrospray ionization58,59. Peptides were identified by searching against a specified database containing 41,407 mRNA sequences using a MS/MS data interpretation algorithm within Mascot. A peptide mass tolerance of 2 ppm and fragment mass tolerance of 0.02 Da were allowed. When the Mascot software was used to search the database, 1,005 proteins were identified, with a false discovery rate (FDR) of less than 1%. Differential expression ratios for proteins were obtained from Mascot software (http://www.matrixscience.com), which calculates protein ratios using only ratios from the spectra that are distinct for each protein and excluding the shared peptides of protein isoforms. To calculate differential expression ratios, all identified spectra from a protein were used to obtain an average protein ratio relative to the control label (i.e., fold change). Student’s t-test was used to analyze the differential expression of proteins between diapause and non-diapause locust eggs. The P-value was calculated using the confidence intervals from the error factor generated in Mascot as
where N is the number of peptide ratios, s is the standard deviation and x represents the mean of the peptide ratios. In this study, we used P ≤0.05 and fold change >1.2 or <0.8 as the thresholds to judge the significance level of differentiated protein expression60.
GO Classification of Differentially Expressed RNA and Proteins and Pathway Analysis
Functional annotation of transcripts and proteins identified in locust egg samples was carried out using Blast2GO, an integrated GO annotation and data mining tool that assigns gene ontology through BLAST searches against nucleotide and/or protein databases61. GO enrichment analysis provides all GO terms that are significantly enriched for differentially expressed genes and proteins in comparison to locust eggs. This method first maps all differentially expressed genes and proteins to GO terms in the database (http://www.geneontology.org/), calculates gene numbers for every term, then uses a hypergeometric test to find significantly enriched GO terms for differentially expressed genes and proteins compared to a locust egg transcriptome/proteome background. The formula used in this calculation is
where N is the number of all genes or proteins with a GO annotation; n is the number of differentially expressed genes or proteins in N; M is the number of all genes or proteins that are notated to the given GO term; and m is the number of differentially expressed genes or proteins in M. The calculated P-value was subjected to a Bonferroni Correction, taking a corrected P-value of 0.05 as a threshold. GO terms fulfilling this condition were defined as significantly enriched for differentially expressed genes or proteins. All identified transcripts and proteins were mapped to a pathway in the Kyoto Encyclopedia of Genes and Genomes (KEGG) database62. Significantly enriched metabolic pathways or signal transduction pathways containing differentially expressed genes and proteins were identified using the same formula as in GO analysis. Here N represents the number of all genes or proteins with KEGG annotation, n is the number of differentially expressed genes or proteins in N, M is the number of all genes or proteins annotated to specific pathways and m is number of differentially expressed genes or proteins in M.
Correlation between protein and mRNA expression
To assess the correlation between transcriptomic and proteomic platforms, we first designated cutoff values to select subsets of genes and proteins with distinctive expression signals. All protein sequences identified by iTRAQ were analyzed and loaded into a searchable database. For each protein, we queried the RNA-seq data for expression patterns of matching transcripts (P-value < 0.05). The significance level of the overlap between detected proteins and transcripts was determined using Pearson’s Chi-squared test with Yates’ continuity correction63.
Additional Information
How to cite this article: Tu, X. et al. Transcriptomic and proteomic analysis of pre-diapause and non-diapause eggs of migratory locust, Locusta migratoria L. (Orthoptera: Acridoidea). Sci. Rep. 5, 11402; doi: 10.1038/srep11402 (2015).
Accession codes: Locust eggs transcriptome datasets are available at NCBI project PRJNA271501 with accession number SRP051668 and SRA with accession number SRR1738245, SRR1738246. Locust eggs proteome datasets are available at Peptide Atlas under a submission number PASS00694.
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Acknowledgements
This research was supported by the earmarked fund for China Agriculture Research System (CARS-35-07) and the Special Fund for Agro-scientific Research in the Public Interest (201003079), P.R. China.
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Z.H.Z. designed the experiments. X.B.T. and J.W. performed the experiments. K.H. analyzed the data. Y.L.F. and G.C.C provided technical and material support. Z.H.Z., X.B.T. and D.W.W. wrote the manuscript. All authors reviewed and considered the manuscript.
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Tu, X., Wang, J., Hao, K. et al. Transcriptomic and proteomic analysis of pre-diapause and non-diapause eggs of migratory locust, Locusta migratoria L. (Orthoptera: Acridoidea). Sci Rep 5, 11402 (2015). https://doi.org/10.1038/srep11402
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DOI: https://doi.org/10.1038/srep11402
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