Ming. cDNAs were transcribed using the SuperScriptTMII reverse transcriptase (Invitrogen) in accordance with the supplier’s instructions using 1 mg of polyA+ mRNAs. The efficiency of each reverse transcription reaction was tested by amplifying the obtained cDNAs with the different primers sets used in the following qPCR reactions using the UptiTherm DNA polymerase (Uptima). The qPCR reactions were performed for each cDNA sample using the qPCR MasterMix Plus for SYBRH Green I No Rox (Eurogentec, Belgium) on a DNA Engine OpticonH2 instrument (Bio-Rad) with the following qPCR conditions : 50uC for 2 min, 95uC for 7 min, 406(95uC for 30 sec, 60uC for 30 sec, 72uC for 45 sec) and specific primers (Table S1). An internal fragment of the Rpl7 ribosomal protein of A. pisum (Genbank accession NM001135898) was used as a control to normalize the for expression (Followed by infection with Lm-gp61 one day later. Following Lm-gp61 infection RPL7-2QPCR Forward: ACTGTTCAGATTGCGTCAGATC, RPL7 -2QPCR reverse: AGTTCCCTTACGCTCTTCAAGT). All reactions were carried out in triplicates for each cDNA prepared from at least four independent mRNA extractions. Quantification of relative mRNA levels was calculated using the DDCt method [22]. The mean and standard error were calculated for each experimental condition.Cloning of the A. pisum foraging genePolyA+ mRNAs were extracted from 100 mg of whole homogenized Acyrthosiphon pisum wingless viviparous adult females using the Micro mRNA purification kit (GE Healthcare). Specific cDNAs were amplified using 0.5 mg of polyA+ mRNA according TM to the BD Smart RACE cDNA amplification kit followed by the TM 2 PCR Enzyme System protocol (BD BiosciBD Advantage ences) with specific primers designed from an EST sequence available in the AphidBase (www.aphidbase.com) and encoding a partial for cDNA (sense primer : GAGTGGAGGTGAGCAGAG, antisense primer : CACTTTTCCGGAGGTCATAG). These primers match with a region of the first tandem cGMP-binding motif of the for gene. Amplified fragments were cloned with the TA CloningH kit (Invitrogen) using the pCRH2.1 vector and transformed into electrocompetent One shotH TOP10 E. coli cells (Invitrogen). Recombinant plasmids from positive clones were extracted, purified and sequenced by GATC Biotech (Konstanz, Germany). The obtained sequences were tested for homology with known for genes using NCBI database. Two sequences homologous to for were then identified and named variant 1 and variant 2. Primers were designed from these two sequences to amplify the corresponding full length cDNAs from freshly extracted polyA+ mRNA samples (variant 1 mRNA sense primer :The Pea Aphid foraging GeneThe In the lung.Materials and Methods SubjectsA total of 296 patients with values obtained for expression levels were relative and could only be compared within each experimental run. Statistical analyses were performed using a one-way ANOVA followed by a Fisher’s PLSD (Protected Least Significant Difference) to test for significant differences of expression between developmental stages or behavioral variants.PKG enzyme activity assaysPKG enzyme activity assays were performed using the Cyclex cyclic GMP dependent protein kinase (cGK) assay kit from Cyclex Co, Ltd. Fresh whole bodies and cut heads from the different behavioral variants were separately homogenized on ice in the provided kinase buffer. Samples were centrifuged for 5 min and supernatants were quantified for total protein amount using the Coo protein assay reagent (Uptima) by the Bradford method. 5 mg of total proteins were then analyzed for PKG enzyme activity, with the following controls to ensure.Ming. cDNAs were transcribed using the SuperScriptTMII reverse transcriptase (Invitrogen) in accordance with the supplier’s instructions using 1 mg of polyA+ mRNAs. The efficiency of each reverse transcription reaction was tested by amplifying the obtained cDNAs with the different primers sets used in the following qPCR reactions using the UptiTherm DNA polymerase (Uptima). The qPCR reactions were performed for each cDNA sample using the qPCR MasterMix Plus for SYBRH Green I No Rox (Eurogentec, Belgium) on a DNA Engine OpticonH2 instrument (Bio-Rad) with the following qPCR conditions : 50uC for 2 min, 95uC for 7 min, 406(95uC for 30 sec, 60uC for 30 sec, 72uC for 45 sec) and specific primers (Table S1). An internal fragment of the Rpl7 ribosomal protein of A. pisum (Genbank accession NM001135898) was used as a control to normalize the for expression (RPL7-2QPCR Forward: ACTGTTCAGATTGCGTCAGATC, RPL7 -2QPCR reverse: AGTTCCCTTACGCTCTTCAAGT). All reactions were carried out in triplicates for each cDNA prepared from at least four independent mRNA extractions. Quantification of relative mRNA levels was calculated using the DDCt method [22]. The mean and standard error were calculated for each experimental condition.Cloning of the A. pisum foraging genePolyA+ mRNAs were extracted from 100 mg of whole homogenized Acyrthosiphon pisum wingless viviparous adult females using the Micro mRNA purification kit (GE Healthcare). Specific cDNAs were amplified using 0.5 mg of polyA+ mRNA according TM to the BD Smart RACE cDNA amplification kit followed by the TM 2 PCR Enzyme System protocol (BD BiosciBD Advantage ences) with specific primers designed from an EST sequence available in the AphidBase (www.aphidbase.com) and encoding a partial for cDNA (sense primer : GAGTGGAGGTGAGCAGAG, antisense primer : CACTTTTCCGGAGGTCATAG). These primers match with a region of the first tandem cGMP-binding motif of the for gene. Amplified fragments were cloned with the TA CloningH kit (Invitrogen) using the pCRH2.1 vector and transformed into electrocompetent One shotH TOP10 E. coli cells (Invitrogen). Recombinant plasmids from positive clones were extracted, purified and sequenced by GATC Biotech (Konstanz, Germany). The obtained sequences were tested for homology with known for genes using NCBI database. Two sequences homologous to for were then identified and named variant 1 and variant 2. Primers were designed from these two sequences to amplify the corresponding full length cDNAs from freshly extracted polyA+ mRNA samples (variant 1 mRNA sense primer :The Pea Aphid foraging GeneThe values obtained for expression levels were relative and could only be compared within each experimental run. Statistical analyses were performed using a one-way ANOVA followed by a Fisher’s PLSD (Protected Least Significant Difference) to test for significant differences of expression between developmental stages or behavioral variants.PKG enzyme activity assaysPKG enzyme activity assays were performed using the Cyclex cyclic GMP dependent protein kinase (cGK) assay kit from Cyclex Co, Ltd. Fresh whole bodies and cut heads from the different behavioral variants were separately homogenized on ice in the provided kinase buffer. Samples were centrifuged for 5 min and supernatants were quantified for total protein amount using the Coo protein assay reagent (Uptima) by the Bradford method. 5 mg of total proteins were then analyzed for PKG enzyme activity, with the following controls to ensure.