Id development.Results The Acyrthosiphon pisum foraging geneTo isolate A. pisum for cDNAs, we designed primers from an A. pisum EST fragment available on the Aphidbase 1.0 database that showed unambiguous homology with the Drosophila melanogaster for gene. 3′ and 5′ RACE experiments resulted in the cloning of two full-length cDNA sequences we named Apfor1 (GeneBank accession number JN812212) and Apfor2 (GeneBank accession number JN812213). Thanks to the recent sequencing of the pea aphid genome, we managed to locate these two complete A. pisum for cDNAs on a genomic scaffold (Scaffold409, GeneBank accession number GL350029) and subsequently deduced that they are composed of 16 exons, exons 3 to 16 being common to Apfor1 and Apfor2 (MedChemExpress I-BRD9 Figure 1). The full size of the Apfor genomic sequence is difficult to determine because of the large size of some introns (notably intron 3 covering more than 300 kb) and of residual sequencing errors. In agreement with genome sequence data, a Emixustat (hydrochloride) site Southern blot analysis clearly showed that only one geneFigure 1. Structure of the Apfor1 and Apfor2 transcripts. Exons 3?6 are identical, only exons 1 and 2 differs as the result of alternative splicing. Scaffold 409 containing the two transcripts is represented at the top. Exons are indicated by grey boxes and introns by dotted lines. White triangles indicate the position of start codons, black triangles indicate the position of the stop codon. doi:10.1371/journal.pone.0065104.gThe Pea Aphid foraging GeneApfor transcripts (Figure S2) we failed to clone probably because of their weak expression.Comparative expression of Apfor among behavioral variants of pea aphid adultsUnder crowded conditions, different behavioral variants are observed in wingless adults, in addition to the typical production of winged morphs able to disseminate over a long distance [1,5]. Indeed, some wingless aphids keep on feeding on the phloem sap under the leaves or on the stems (variants VWLc) while others leave the plant, walk and forage their environment to find better conditions for feeding and producing offspring (variants VWLf). We thus analyzed the level of both Apfor transcripts in four categories of behavioral adult variants, three reared under high population density (winged adults VW, wingless sedentary crowded adults VWLc and wingless forager adults VWLf) and one reared under low population density (wingless sedentary adults VWL) (Figure 3). The expression of the Apfor1 transcript is significantly higher in the VWLc variants compared to other variants (one-way ANOVA followed by Fisher’s PLSD test; F = 8,71, P,0,001) (Figure 3A). Apfor2 transcripts are also significantly more expressed in the VWLc variant (F = 4,08, P,0,05) but we observe the same trend in the VWLf variant. A higher standard error value is observed for both variants (Figure 3B). These results confirm our previous observations (Figure 2) that no significant difference occurs in Apfor expression between VW reared under high population density and VWL reared under low population density. So, the high expression level of the pea aphid for gene seems to be associated with the exploratory behavior due to crowded conditions rather than with morphological variants.PKG enzyme activity among behavioral variants of pea aphid adultsPKG enzyme activities, that represent at least the combined activities of the two Apfor variants, were comparatively measured in the different behavioral variants from whole bodies or heads. Figure 4.Id development.Results The Acyrthosiphon pisum foraging geneTo isolate A. pisum for cDNAs, we designed primers from an A. pisum EST fragment available on the Aphidbase 1.0 database that showed unambiguous homology with the Drosophila melanogaster for gene. 3′ and 5′ RACE experiments resulted in the cloning of two full-length cDNA sequences we named Apfor1 (GeneBank accession number JN812212) and Apfor2 (GeneBank accession number JN812213). Thanks to the recent sequencing of the pea aphid genome, we managed to locate these two complete A. pisum for cDNAs on a genomic scaffold (Scaffold409, GeneBank accession number GL350029) and subsequently deduced that they are composed of 16 exons, exons 3 to 16 being common to Apfor1 and Apfor2 (Figure 1). The full size of the Apfor genomic sequence is difficult to determine because of the large size of some introns (notably intron 3 covering more than 300 kb) and of residual sequencing errors. In agreement with genome sequence data, a Southern blot analysis clearly showed that only one geneFigure 1. Structure of the Apfor1 and Apfor2 transcripts. Exons 3?6 are identical, only exons 1 and 2 differs as the result of alternative splicing. Scaffold 409 containing the two transcripts is represented at the top. Exons are indicated by grey boxes and introns by dotted lines. White triangles indicate the position of start codons, black triangles indicate the position of the stop codon. doi:10.1371/journal.pone.0065104.gThe Pea Aphid foraging GeneApfor transcripts (Figure S2) we failed to clone probably because of their weak expression.Comparative expression of Apfor among behavioral variants of pea aphid adultsUnder crowded conditions, different behavioral variants are observed in wingless adults, in addition to the typical production of winged morphs able to disseminate over a long distance [1,5]. Indeed, some wingless aphids keep on feeding on the phloem sap under the leaves or on the stems (variants VWLc) while others leave the plant, walk and forage their environment to find better conditions for feeding and producing offspring (variants VWLf). We thus analyzed the level of both Apfor transcripts in four categories of behavioral adult variants, three reared under high population density (winged adults VW, wingless sedentary crowded adults VWLc and wingless forager adults VWLf) and one reared under low population density (wingless sedentary adults VWL) (Figure 3). The expression of the Apfor1 transcript is significantly higher in the VWLc variants compared to other variants (one-way ANOVA followed by Fisher’s PLSD test; F = 8,71, P,0,001) (Figure 3A). Apfor2 transcripts are also significantly more expressed in the VWLc variant (F = 4,08, P,0,05) but we observe the same trend in the VWLf variant. A higher standard error value is observed for both variants (Figure 3B). These results confirm our previous observations (Figure 2) that no significant difference occurs in Apfor expression between VW reared under high population density and VWL reared under low population density. So, the high expression level of the pea aphid for gene seems to be associated with the exploratory behavior due to crowded conditions rather than with morphological variants.PKG enzyme activity among behavioral variants of pea aphid adultsPKG enzyme activities, that represent at least the combined activities of the two Apfor variants, were comparatively measured in the different behavioral variants from whole bodies or heads. Figure 4.
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