Background

Ancient and now highly specialized associations with bacterial symbionts are widespread in invertebrate groups that feed on nutrient-poor diets [1]. Such associations are common in insects, in which the best studied symbiotic system is that of aphids (Insecta: Hemiptera: Aphididae) and their primary symbiont Buchnera aphidicola [2]. Buchnera, which has not been established in laboratory cultures, inhabits specialized host cells (bacteriocytes), is required for nutrition (host development, growth and reproduction) and has been strictly vertically transmitted from mother to offspring for the last 150 million years [25]. In addition to being the best studied insect-symbiont system [6], aphids are of general interest due to their economic and agricultural status as plant pests and plant disease vectors [7] and their complex life cycles with multiple developmental pathways and parthenogenesis [8, 9].

The pea aphid Acyrthosiphon pisum (Insecta: Hemiptera: Aphididae) will be one of the first insect species outside of the Holometabola to serve as a model system in genomics [10]. Currently, little is known about gene expression in this newly emerging model organism. In addition, it is already clear from the growing collection of aphid ESTs that aphids possess many genes that are absent from Drosophila and other holometabolous insect taxa [1113]. Accurate and successful interpretation of the A. pisum genome sequence will depend critically on studies of gene expression under different environmental conditions, in different tissues and morphs, and at different developmental stages [14, 15].

The complete genome sequences are now available for the Buchnera from three aphid species [5, 16, 17], including A. pisum [5]. Facilitated by these genome sequences and other studies, Buchnera has become a model for studying the evolution of symbiotic and pathogenic lifestyles in bacteria [6, 18, 19].

In the present study we take a metagenomic approach [20] to examining transcriptional responses to heat shock in a host/symbiont system, using pooled RNA samples and a microarray containing gene sets from both organisms. Select results were verified with reverse-transcriptase quantitative PCR (RT-qPCR). To our knowledge, this dual-genome microarray is the first used to examine simultaneously the pooled transcriptome of an animal host and its symbiont; a previous dual-genome array has been used to study Rhizobium-plant interactions [21].

The transcriptional response to heat shock has been well characterized in other Buchnera [22] and in other insects [23], enabling us to generate a priori predictions and thus to assess the success of our array design. Further, aphids are highly sensitive to heat, with considerable variation among species (e.g., [2427]). Part of this sensitivity stems from the intolerance of the resident symbionts to high temperature. Aphid lineages can be rendered infertile as a consequence of heat-induced elimination of their resident Buchnera [28], and field populations of A. pisum exposed to naturally occurring high temperatures undergo a decline in the number of bacteriocytes, reflecting the decline of the Buchnera population within heat-stressed aphid hosts [29]. Thus, the overall thermal tolerance of this symbiotic system is dependent on both host and symbiont responses to thermal challenge.

To date, there are no published studies on heat shock responses of any aphid genes. Previously, Wilcox et al. [22] studied gene expression under heat shock in Buchnera derived from the aphid Schizaphis graminum and identified a set of nine genes that were significantly upregulated. Six of the nine genes, mopA (= groEL), mopB (= groES), dnaJ, dnaK, grpE, and ibpA are heat shock genes in other bacteria such as the related species Escherichia coli and are known to function in the recycling and refolding of degraded proteins. Two additional genes, fpr and the pseudogene of yjeA, showed elevated transcript levels following heat shock. Both are positioned immediately downstream of ipbA and its σ32 heat shock promoter, and their response reflects transcriptional read-through based on reverse transcriptase quantitative PCR assays of different regions of the transcripts [22].

Results and discussion

Heat shock response in Buchnera of A. pisum

Overall, the set of genes responding to heat shock in the Buchnera of A. pisum is similar to the set previously identified in the Buchnera of S. graminum [22]. In both, the following genes belonging to the E. coli heat shock (HS) regulon were significantly upregulated: dnaK, mopA (= groEL), mopB (= groES), ibpA and dnaJ (Figure 1A). (We also detected a similar fold-change in expression of the E. coli HS regulon gene, grpE, in Buchnera of A. pisum as reported for Buchnera of S. graminum, but this change was not statistically significant.) In Buchnera of both aphid species, yjeA is downstream of ibpA and fpr, but encoded on the opposite strand. Our results show an increase in yjeA transcript with heat shock in Buchnera of A. pisum, as described for Buchnera of S. graminum. Because the microarray probes consist of double-stranded amplicons, the most likely interpretation is that the heat-shock induced transcription of ibpA continues through both fpr and yjeA, resulting in elevated transcription of the non-coding strand of yjeA (the gene fpr is not present on our array). We verified this explanation for yjeA transcription under HS through targeted RT-PCR of a region overlapping ibpA, fpr, and the complement of yjeA (data not presented), using the same approach applied to Buchnera of S. graminum [22].

Figure 1
figure 1

Fold-change in gene expression after exposure to heat stress. Line at -Log(P) = 5 corresponds to P = 0.0001. A. Buchnera EST1 (dnaK) = CN582666, EST2 (fliI) = CN587517, EST3 (mopA) = CN585306, EST4 (metE) = CN582733. B. Pea aphid, A. pisum. EST5 = CN584139, EST6 (hsp70) = CN586725, EST7 = CF588076, EST8 = CN586853, EST9 = CN585958, EST10 = CF587727, EST11 = CN587624, EST12 = CN584928.

In addition to the heat-responsive genes identified for Buchnera of S. graminum [22], two other Buchnera probes showed increased signal following HS (Figure 1A): EST2 (fliI), flagellum-specific ATP synthase and EST4 (metE), 5-methyltetrahydropteroyltriglutamate-homocysteine S-methyltransferase. The gene metE was present as two types of probe: one, EST4, showed consistent increase in signal under HS, and the other, a directly amplified product from genomic DNA, did not respond. Our interpretation is that the spot corresponding to EST4 was contaminated with some other sequence, and that metE is not responding.

Signal from several Buchnera genes was decreased following HS (Figure 1A). These include aroK, mraY, cysJ, carA and cysQ. Of these, carA also showed down-regulation under HS in the study of Buchnera of S. graminum [22].

Using RT-qPCR, to investigate the accuracy of our microarray results for a select set of eight Buchnera genes, we found good congruence between methods, using the non-HS genes argG and cysG as controls (Figure 2, data for cysG not shown).

Figure 2
figure 2

Mean fold-change estimates for select Buchnera of A. pisum genes compared between microarray and RT-qPCR methods. Standard error bars are shown. RT-qPCR data have been standardized relative to argG.

While the set of genes responding under HS corresponded to the set identified for Buchnera of S. graminum, the magnitude of response was much larger for Buchnera of A. pisum, both from the microarray and the RT-qPCR estimates. The HS treatment was the same for both studies; yet, expression changes ranged from under 2-fold to 13-fold in Buchnera of S. graminum [22] compared with 5-fold to 70-fold in Buchnera of A. pisum (Figure 1A, Figure 2).

Heat shock response in A. pisum

Two paralogs of the HS gene, hsp70, were included on the array, one derived from a PCR product amplified from genomic DNA (hsp70) and the other derived from an EST (Figure 1B, EST6 – CN586725). Both showed greater than 16-fold increase in transcript abundance under HS (Figure 1B). Seven other genes (Figure 1B, EST5 and EST7 – EST12) showed large fold-changes and/or statistically significant changes in gene expression under HS conditions.

We investigated the accuracy of our microarray results using RT-qPCR for eight A. pisum genes representing a range of responses on the array. Two of these showed no change on the array and were used as control genes (EST13 (CN587115, a homolog of EF1a) and EST14 (CN582657)), and both control genes gave similar results. We found good congruence between microarray and RT-qPCR methods for aphid EST 6 (a homolog of hsp70) (log2 fold-change estimate from microarray data: 5.67 ± S.E. 0.87 c.f. log2 fold-change estimate from RT-qPCR: 7.32 ± S.E. 1.03). However, RT-qPCR indicated no significant change in relative expression for five of the aphid ESTs that showed either upregulation (EST5, EST7, EST8 and EST10) or down-regulation (EST12) under HS. This indicates that expression of the designated gene (corresponding to the EST and to the sequence matching the PCR primers), does not change under HS. Two explanations are (1) that a paralogous gene is undergoing change in expression giving cross-hybridization on the array but not giving PCR product because of the greater stringency of the RT-qPCR and (2) that there is contamination of the arrayed spots attributable to splash during transfers to the microtiter plates or carry-over of the array pins.

To discriminate between these two possibilities, we performed a dye-flip microarray hybridization experiment using samples differing only in the presence or absence of added amplicons of known HS genes represented on the array. RNA representing the transcript pool of aphids under control conditions was divided into two portions, one spiked with amplicons of four upregulated Buchnera genes (dnaK, ibpA, mopA, yjeA) and one spiked with the amplicon of an upregulated aphid gene (hsp70). Two of the five aphid genes that showed incongruent results (EST8 and EST10) did not change expression in the spike experiment. This indicates that the observed microarray results from the HS experiment cannot be explained as the result of contamination among probes on the array. Instead, they likely reflect cross-hybridization of closely related gene transcripts [30].

Non-target sequences with >70% sequence identity can cross-hybridize to cDNA probes [31]. This is illustrated on our array, which contains three members of the aphid hsp70 gene family; hsp70, which was amplified using PCR primers from genomic DNA for inclusion on this array and for which we have a cloned PCR product; EST6, which was isolated from EST libraries (Figure 1) and EST15 (CN584562), which shows homology to hsp70 and hsp68 from other insect taxa and did not show significant upregulation under HS conditions (Table 1). PCR primers designed to EST6 do not amplify our cloned hsp70 product or EST15; however, in the spike experiment, hsp70 PCR product hybridized to itself and to both the EST6 and EST15 probes (Table 1). Similarly, expression changes in paralogous genes are the most evident explanation for the change in signal of EST8 and EST10 (Table 1). The final two aphid ESTs, EST5 and EST7, did show significant "upregulation" in the spiked pools (Table 1). The EST5 probe cross-hybridized with hsp70 and the EST7 probe with one of the four Buchnera genes. We could not find any significant stretches of sequence similarity to explain these results, suggesting that these probes were contaminated. The EST5 and EST7 results are most readily attributable to splash on the microtiter plates. However, results from the spike experiment (Table 1) clearly indicate that apparent upregulation of wg, wnt2 and Dll (fold-changes of 6–12 under HS, without strong statistical significance (Figure 1B)) resulted from pin carryover of the hsp70 probe during the printing process. The same pin stamped hsp70, Dll, wg and wnt2, in that order.

Table 1 Spike microarray hybridization data listing genes showing significant signal increase. Genes that were used to spike the control RNA are marked * for Buchnera genes and ** for the aphid gene. Positive log2 fold-changes indicate genes that cross-hybridized with aphid hsp70 and negative log2 fold-changes indicate genes that cross-hybridized with the Buchnera genes. Genes reported are those that had log2 fold-changes ≥ |1| and a -log(P) ≥ 2. Genes are listed in order of signal strength.

Usefulness of EST-based microarrays for functional annotation of the aphid genome

These results suggest that, in addition to hsp70, paralogs of EST8 and of EST10 undergo significant upregulation under HS. Both have homologs in many other taxa, but we found no reports of involvement in the HS response in other organisms. EST8 shows significant homology to tyrosyl-tRNA synthase from Homo sapiens, Mus musculus and Drosophila virilis, while EST10 is homologous to the gene encoding the molybdenum cofactor of sulfurase in Bombyx mori, Bos taurus and Homo sapiens. Molybdenum cofactor sulfurase is responsible for xanthine dehydrogenase activation in various organisms, a gene which plays a critical role in nitrogen metabolism, especially in insects [32]. Our results suggest that genes that share significant sequence similarity to these two ESTs have a function in the heat stress response in aphids.

Conclusion

One of the outstanding questions in host/symbiont systems is how gene expression in the partner organisms is coordinated. EST studies of aphid bacteriocytes have shown elevated expression of genes associated with a range of cellular functions including amino acid metabolism, cell transport, and antibacterial activity [13]. The presence of these functional categories at high frequency in bacteriocyte EST libraries highlights important aspects of genome coordination between symbiont and host. Further progress in understanding how and when these genes are upregulated and the roles they play in mediating the symbiosis will require extensive expression studies using arrays such as the one we describe here.

We have demonstrated the feasibility of using a dual-genome microarray to simultaneously study the expression profile of an aphid and its obligate bacterial symbiont. The success of this approach is dependent on the relative abundances of transcripts from the partner organisms. Buchnera occurs in large numbers within aphids; their genomes constitute about 5–10% of total DNA content [3]. A quantitative PCR study of gene copy number in intact adult pea aphids indicated a ratio of approximately 7.5 single copy Buchnera genes for each single copy aphid gene (H. Dunbar and N. Moran, unpublished data). This estimate is consistent with previous estimates of genome sizes of the two organisms and of the proportion of total DNA belonging to Buchnera [3]. Thus, we expected transcript abundances of Buchnera and aphid genes to be comparable, enabling hybridization of the pooled sample on the same array without loss of signal for either organism. Use of a dual-genome array for the study of symbiosis in systems where symbionts are found in low copy number, e.g. Wolbachia, the facultative bacterial endosymbiont of Drosophila and other insects [33], is likely to prove more difficult. However, many animals, including many other insects and marine invertebrates, do possess large numbers of obligate primary symbionts. In these composite organisms, an understanding of the integration of component genomes requires the synchronous examination of gene expression in each member.

Finally, our results for the pea aphid genes suggest that the pea aphid genome may contain many gene paralogs that are differentially regulated. Preliminary analysis from an EST project suggests that the pea aphid genome may contain many gene duplications [34]. This fact will complicate analysis of differential gene expression in pea aphids using cDNA microarrays, and suggests that establishing the differential regulation of specific genes will require qPCR. The full extent of gene paralogy in the pea aphid will soon be revealed by whole genome sequencing [10].

Methods

Microarray design

We designed a 7,448 spot, dual-genome microarray containing 1,862 genes. The array includes 76 Buchnera genes representing the E. coli heat shock (HS) regulon (clpX, dnaJ, dnaK, grpE, hflB, hslU, hslV, htpX, htrA, ibpA, mopA and mopB), essential amino acid biosynthesis genes (argA, argB, argC, argD, argE, argF, argG, argH, aroA, aroB, aroC, aroD, aroE, aroH, aroK, carA, carB, cysD, cysG, cysH, cysI, cysJ, cysK, cysN, cysQ, dapA, dapB, dapD, dapE, dapF, glyA, hisB, hisC, hisD, hisF, hisI, ilvC, ilvH, ilvI, leuA, leuD, lysA, metE, pheA, thrA, thrB, trpA, trpC and trpG) and a number of other genes representative of various functional categories such as cold shock, cell wall biosynthesis and DNA repair (cspC, cysS, endA, lgt, mraY, mrcB, mrsA, murC, murE, murF, nlpD, prfB, serC, ung and yjeA). The array also includes, nine aphid developmental and heat shock genes (distal-less, eyeless, fused, nanos, vasa, vasa-like, wingless, wnt2 and hsp70) and 1777 A. pisum ESTs (GEO Accession: GSE3742). All Buchnera genes were amplified using gene-specific primers designed from the Buchnera of A. pisum genomic sequence (GenBank Accession: BA000003, [6]). Primers were designed, where gene length permitted, to give an optimal product of 1000 base pairs with a melting temperature of 55°C. If gene coding sequences were less than 1000 base pairs, primers were designed to maximize product length. We amplified Buchnera genes in two 50 μl PCR reactions from a laboratory line of A. pisum. This line, 7-2-1 was collected in August 2001 in Cayuga County, New York from alfalfa by Jacob Russell. Since its collection, 7-2-1 has been maintained in continuous parthenogenetic culture in the laboratory of NAM.

All A. pisum ESTs were derived from a cDNA library constructed in the laboratory of DLS (described in [34], GenBank Accessions: CF587442 - CF588411 and CN582088 - CN587684). ESTs were clustered in a unigene set and 1824 genes were selected for inclusion based primarily on significant tblastx scores to other eukaryotes when used as queries in searches of the GenBank nr database. The corresponding cDNAs were amplified using T3 and T7 primers to pBluescript.

Genes were arranged in duplicate spots on slides, with Buchnera genes grouped into the first and second of 24 subarrays. In addition to spot duplication, the entire set was printed twice on each slide thus; each spot was printed in quadruplicate.

Heat shock

A single isofemale line of A. pisum was used in all HS experiments. This clone, called "TUC", was collected by NAM from fava bean in a garden in Tucson, Arizona in June 1999 and has been maintained in continuous parthenogenetic culture on fava bean at 20°C in the laboratory of NAM since its collection. Clone TUC, in addition to harboring the primary aphid symbiont, Buchnera, is host to the secondary bacterial symbiont, Candidatus Serratia symbiotica, previously known as the "R-type" [35].

Six to ten adult A. pisum were placed on a single fava bean plant in a cup cage and allowed to reproduce at 20°C 16 L:8 D. After 24 – 48 hours the adult aphids were removed from plants and flash-frozen in liquid nitrogen. First generation aphids were then maintained for one week, the developmental period required to attain the adult stage. Heat shock experiments were carried out 1 – 2 days following ecdysis to adulthood. Prior to HS, 10 – 20 control aphids were removed from each plant, flash-frozen in liquid nitrogen and stored at -80°C until RNA extraction and microarray hybridization. Heat shock conditions were applied by ramping from 20°C to 36°C over a two hour period at a rate of 2°C/15 min and then maintaining aphids at 36°C for an additional 2 hours (4 hours in total). At 4 hours cultures were removed from the growth chamber and aphids were quickly collected into Eppendorf tubes, flash-frozen in liquid nitrogen and stored at -80°C until processing. Two biological replicates of clone TUC were exposed to heat shock in parallel.

RNA extraction and microarray hybridization

We extracted total RNA from control and HS samples using an RNeasy Mini Kit (Qiagen Cat. No.74104). RNA quantity and quality was assessed using an RNA LabChip® on the Agilent 2100 Bioanalyzer. We constructed cDNA from 10 μg of total RNA using Omniscript Reverse Transcriptase and reaction buffer (Qiagen), 6 ng random hexamer primers, 0.5 mM each dATP, dCTP, dGTP, 0.3 mM dTTP, and 0.2 mM amino-allyl linked dUTP. RNA was hydrolyzed, and purified cDNA populations were coupled to Cy3 or Cy5 fluors (Amersham). We flipped dye labels between treatments across experimental replicates. Therefore, results from 4 total slides were analyzed. Purified, labeled cDNA populations were suspended in 80 μl Sigma Hybridization Buffer with 20 μg Human COT1 DNA. Microarray slides were rehydrated, UV crosslinked, and denatured immediately before hybridization. Target samples were combined, denatured for 10 min at 94°C, and pipetted into sealed, microvolume slide manifolds. We ran hybridizations in a GeneTAC automated station at 47°C for 16 hours and programmed 3 washes of variable-stringency SDS/SSC solutions (Sigma).

Analysis

Signal intensities were measured using spot-finding software, softWoRx Tracker (version 2.20, MolecularWare Inc). Raw median spot intensity and median background intensity data were exported; median background signal intensities were subtracted from median signal intensities. A zero signal value was substituted for any negative signal intensities and all non-zero values were log2-transformed. In order to compensate for differences in expression levels between the two genomes represented on the array we analyzed each species separately, by normalizing across probes for each genome. For each species we imported log2-transformed data into SAS version 9 and used 'PROC MIXED' to model and remove systematic sources of variation contributed by Cy3 versus Cy5 dyes, slide and hybridization effects, slide × dye interactions and slide × treatment interactions [36, 37]. Statistical residuals generated from the normalization step were subjected to mixed-model analyses of variance (log2 normalized data for this experiment can be accessed at GEO Accession: GSE3742). We regarded as potentially meaningful any response that showed fold-change greater than four or that had P-values less than 0.0001.

Verification of expression with RT-qPCR

We verified microarray results with real-time quantitative PCR from cDNA from both biological replicates used for microarray hybridization for four of the Buchnera genes that appeared to be upregulated under HS conditions (dnaK, ibpA, mopA, and yjeA), two Buchnera genes that did not show a HS response (argG and cysG) and two Buchnera genes that appeared to be down-regulated under HS conditions (aroK and carA) as well as five aphid ESTs that appeared to be upregulated under HS conditions (EST5, EST6: hsp70, EST7, EST8 and EST10, Figure 1b), two aphid genes that did not show a heat shock response (EST13: ef1α and EST14), and one aphid EST that appeared to be down-regulated under HS conditions (EST12, Figure 1b) following the protocol described in [38]. Primers were designed to amplify short regions of these genes and were as follows:

argG: F 5' TTCACTATGTCATGGTGCTACTG 3' and R 5' TGCCAGGAATTTTCATCTTTAC 3'; aroK: F 5' CTGGGAAAAGCACTATTGGTC 3' and R 5' ACCTCCTCCTGTAGCAAGAAC 3'; carA: F 5' TTGCGATTACGCTATTCATGC 3' and R 5' CCTTAACAGGATGGTTGCCTC 3'; cysG: F 5' AGGTGGTGATCCCTTTATTTTC 3' and R 5' GAGTATTTGCGATGTGTCAGTG 3'; dnaK: F 5' ATGGGTAAAATTATTGGTATTG 3' and R 5' ATAGCTTGACGTTTAGCAGG 3'; ibpA: F 5' CCAATATCTGATACACCGAC 3' and R 5' TGAACAGATATATCTAATTCTTTTTC 3'; mopA: F 5' ATGTAAAAGACGGAAAAGG 3' and R 5' CCTGCTGGAGAAGAACTAG 3'; yjeA: F 5' CGAACAAAAAGGTTGATACCATTC 3' and R 5' TTATTAGCATCAGAAAGCGGATC 3'; EST13 – ef1α: F 5' CTGATTGTGCCGTGCTTATTG 3' and R 5' TATGGTGGTTCAGTAGAGTCC 3'; EST6 – hsp70: F 5' TAAGAGGAAAACTAAAAAGGACG 3' and R 5' GGAAACTCGGGTGTAGAAATC 3'; EST14: F 5' TATGTTGCAGCAGCCGATAC 3' and R 5' AATGCTGGTCCTTCAGATGC 3'; EST5: F 5' CAAGAAATTCTCCCCTCATTTG 3' and R 5' TGCTCTTGCTAACCCACCAC 3'; EST7: F 5' TTCAAATCGTCGAAGTGTGC 3' and R 5' AAGTCGTCGACCGTGATTTC 3'; EST8: F 5' GCTGTTCTGCGTTCACTTGTAC 3' and R 5' AGTCCGCTATTTTGGATATTGG 3'; EST10 F 5' TTTGGAAGGAATGGACTGTGG 3' and R 5' TTGAGCGTTGATTGTGTGGAC 3'; EST12: F 5' GAAAGAAGATTTGGTGCTTGG 3' and R 5' CTATTATGGGCACTTGCGATC 3'.

Verification of spot identity with select resequencing across the array

Spots that showed a > 4 fold-change (log2 fold-change = ± 2) and/or a significant fold-change (≥ -Log(P) = 5), together with the set of ESTs that we annotated through blast-searching as HS genes were resequenced using vector primer, T3, to confirm spot identity. The identity of the majority of resequenced spots (24/36 spots) was verified by a blastn search restricted to the NCBI "EST_other" database [39], which includes the EST sequences for the fragments on our array. A subset of resequenced spots (11/36 spots) returned poor sequence, as expected if more than one template was present. However, three of these, CN585306 (EST3, Buchnera mopA), CN586357 (aphid dnaJ) and CN586725 (EST6, aphid hsp70), were annotated as HS genes and showed large and significant upregulation under HS conditions. The correspondence between gene annotation and change in expression for these genes indicates that the expected gene is present on the array in the correct position. This observation indicates that most elements on the array contain the correct sequence.

Investigation of cross-hybridization of heat-shock gene products

We investigated cross-hybridization of the most upregulated heat shock genes on our array by spiking control RNA with labeled PCR products corresponding to HS genes. Four Buchnera genes (dnaK, ibpA, mopA and yjeA) and one aphid gene (hsp70) were amplified. PCR reactions were carried out for each gene in two 25 μl volumes containing 50 mM KCl, 10 mM Tris-HCl, 1.5 mM Mg2+, 2.5 mM of each dATP, dCTP and dGTP, 1 mM dTTP, 1.5 mM amino-allyl linked dUTP (Sigma A0410-1MG), 0.25 units of Eppendorf Taq DNA polymerase and 10 ng of DNA (Buchnera genes) or cDNA (EST6 – hsp70). Primers used to amplify genes selected for spiking were as follows: Buchnera of A. pisum dnaK: F 5' CACCAGAGAGAACTCCTCCC 3' and R 5' ATGGATGGCAATAAACCACG 3', Buchnera of A. pisum ibpA: F 5' TCAATTAACACTAAGTATTCCTGG 3' and R 5' TAGGTTTTTCCTCTTCCGG 3', Buchnera of A. pisum mopA: F 5' ACCACAACAGCAACATTATTAGC 3' and R 5' ACCTCCAGCAACTACACCTTC 3', Buchnera of A. pisum yjeA: F 5' GAAGCGTTTATTAGCATCAG 3' and R 5' TGAACAAGGAGGTAAGCC 3', A. pisum hsp70: F 5' GTGTTGATATTTGACCTGGGC 3' and R 5' AATGGTAGAGTTGCGTTCGAC 3'.

We performed a standard dye-flip hybridization experiment using RNA isolated from a control line and spiked with either 20 ng of the aphid hsp70 PCR product or 20 ng of each of the four Buchnera gene PCR products. Spikes were added to the RNA samples following generation of cDNA and prior to cy3 and cy5 labelling. Thus, for one hybridization, the aphid spike was cy3 labeled and the Buchnera spikes were cy5 labeled and for the second hybridization the dyes were reversed. In this way we were able to distinguish between spots that were cross-hybridizing with aphid hsp70 versus the Buchnera genes. Data from the spike array hybridization experiment were analyzed using the analysis pipeline described above for the heat shock experiments.