H lane and immunoblotted with polyclonal anti-human b2-m antibody (Dako). (D) Representative dot blot developed by antibody recognizing Chebulagic acid oligomers (A11) in transgenic worms and (E) quantification of A11-immunoreactive bands. Data are expressed as mean of density of A11 immunoreactive bands/mg of protein 6 SE of three independent experiments (N = 9); *p,0.01 vs WT, according to one-way ANOVA. doi:10.1371/journal.pone.0052314.gtherefore the growth rate is constant within larval phases and, reached a plateau in late adulthood [28]. After synchronization, the numbers of worms were MedChemExpress 307538-42-7 scored after 24, 48 and 72 hours that correspond to the L1/L2, L2/L3 and L4/adult larval stages, respectively. WT nematodes exhibited a constant number of worms and a constant growth rate similarly to that observed in animals transfected with the empty vector (Figure 4A). In P32G and DN6 transgenic C. elegans strains, the percentage of worms AZ-876 site reaching the L1/L2 stage was JI 101 web significantly reduced than in WT (83.3 for WT and 27.6 and 37.8 for P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA). The irregular growth rate buy ML-281 compared to WT was also observed at the L2/L3 larval stage (81.4 for WT and 20.0 and 18.7 P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA, Figure 4A). This resulted in a significant reduction in the percentage of worms reaching the adulthood, being the 88.6 for WT nematodes and 13.8 and 22.9 for P32G and DN6 transgenic animals, respectively (p,0.01vs. WT, One-way ANOVA) and indicates that the expression of the mutated or truncated isoforms of the protein affected the nematodes growth and development. The phenotypic abnormality well correlated with the aggregation pathway of b2-m. In particular, a correlation coefficient ofR = 0.979 was determined when the percentage of transgenic worms reaching the adulthood, 72 hours after synchronization, was plotted with the amount of A11-positive oligomeric assemblies detected by dot blotting (Figure 4B). To determine whether b2-m affected the health of nematodes and their lifespan, the overall nematodes survival was evaluated. The expression of wild type b2-m significantly decreased the median lifespan of transgenic worms compared to nematodes injected with the empty vector (Figure 4C, median survival respectively: 13 days and 10 days for Vector and WT, p,0.05, Wilcoxon test). The insertion of both the P32G mutated gene and deleted DN6 sequence similarly shortened the survival of worms by 38 compared to the empty vector (median of survival: 8 days for both P32G and DN6, p,0.001 vs. Vector, Wilcoxon test) and by 20 compared to WT (p,0.01, Wilcoxon test). Thus, nematodes expressing the mutated or truncated gene had a shorter lifespan, MedChemExpress Lixisenatide indicating that, in vivo, P32G and DN6 show a greater proteotoxicity than WT b2-m. The presence of misfolded proteins in body wall muscle cells can induce dysfunctions in the coordination and motility of C. elegans [6].C. elegans Models for b2-m AmyloidosisFigure 3. Localization of b2-m in transgenic C. elegans strains. Overlay of bright field and immunofluorescence images of head, vulva and tail of transgenic C. elegans strains. All animals depicted are 2 days adult worms. A specific b2-m related signal (red, using a polyclonal anti human b2-m antibody) was observed at the vulva muscles and anal sphincter muscle in the tail (red arrows) whereas no signal was observed in the head muscles. Scale bar, 50 mm. doi:10.1371/journal.pone.0052314.gWe investigated whether.H lane and immunoblotted with polyclonal anti-human b2-m antibody (Dako). (D) Representative dot blot developed by antibody recognizing oligomers (A11) in transgenic worms and (E) quantification of A11-immunoreactive bands. Data are expressed as mean of density of A11 immunoreactive bands/mg of protein 6 SE of three independent experiments (N = 9); *p,0.01 vs WT, according to one-way ANOVA. doi:10.1371/journal.pone.0052314.gtherefore the growth rate is constant within larval phases and, reached a plateau in late adulthood [28]. After synchronization, the numbers of worms were scored after 24, 48 and 72 hours that correspond to the L1/L2, L2/L3 and L4/adult larval stages, respectively. WT nematodes exhibited a constant number of worms and a constant growth rate similarly to that observed in animals transfected with the empty vector (Figure 4A). In P32G and DN6 transgenic C. elegans strains, the percentage of worms reaching the L1/L2 stage was significantly reduced than in WT (83.3 for WT and 27.6 and 37.8 for P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA). The irregular growth rate compared to WT was also observed at the L2/L3 larval stage (81.4 for WT and 20.0 and 18.7 P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA, Figure 4A). This resulted in a significant reduction in the percentage of worms reaching the adulthood, being the 88.6 for WT nematodes and 13.8 and 22.9 for P32G and DN6 transgenic animals, respectively (p,0.01vs. WT, One-way ANOVA) and indicates that the expression of the mutated or truncated isoforms of the protein affected the nematodes growth and development. The phenotypic abnormality well correlated with the aggregation pathway of b2-m. In particular, a correlation coefficient ofR = 0.979 was determined when the percentage of transgenic worms reaching the adulthood, 72 hours after synchronization, was plotted with the amount of A11-positive oligomeric assemblies detected by dot blotting (Figure 4B). To determine whether b2-m affected the health of nematodes and their lifespan, the overall nematodes survival was evaluated. The expression of wild type b2-m significantly decreased the median lifespan of transgenic worms compared to nematodes injected with the empty vector (Figure 4C, median survival respectively: 13 days and 10 days for Vector and WT, p,0.05, Wilcoxon test). The insertion of both the P32G mutated gene and deleted DN6 sequence similarly shortened the survival of worms by 38 compared to the empty vector (median of survival: 8 days for both P32G and DN6, p,0.001 vs. Vector, Wilcoxon test) and by 20 compared to WT (p,0.01, Wilcoxon test). Thus, nematodes expressing the mutated or truncated gene had a shorter lifespan, indicating that, in vivo, P32G and DN6 show a greater proteotoxicity than WT b2-m. The presence of misfolded proteins in body wall muscle cells can induce dysfunctions in the coordination and motility of C. elegans [6].C. elegans Models for b2-m AmyloidosisFigure 3. Localization of b2-m in transgenic C. elegans strains. Overlay of bright field and immunofluorescence images of head, vulva and tail of transgenic C. elegans strains. All animals depicted are 2 days adult worms. A specific b2-m related signal (red, using a polyclonal anti human b2-m antibody) was observed at the vulva muscles and anal sphincter muscle in the tail (red arrows) whereas no signal was observed in the head muscles. Scale bar, 50 mm. doi:10.1371/journal.pone.0052314.gWe investigated whether.H lane and immunoblotted with polyclonal anti-human b2-m antibody (Dako). (D) Representative dot blot developed by antibody recognizing oligomers (A11) in transgenic worms and (E) quantification of A11-immunoreactive bands. Data are expressed as mean of density of A11 immunoreactive bands/mg of protein 6 SE of three independent experiments (N = 9); *p,0.01 vs WT, according to one-way ANOVA. doi:10.1371/journal.pone.0052314.gtherefore the growth rate is constant within larval phases and, reached a plateau in late adulthood [28]. After synchronization, the numbers of worms were scored after 24, 48 and 72 hours that correspond to the L1/L2, L2/L3 and L4/adult larval stages, respectively. WT nematodes exhibited a constant number of worms and a constant growth rate similarly to that observed in animals transfected with the empty vector (Figure 4A). In P32G and DN6 transgenic C. elegans strains, the percentage of worms reaching the L1/L2 stage was significantly reduced than in WT (83.3 for WT and 27.6 and 37.8 for P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA). The irregular growth rate compared to WT was also observed at the L2/L3 larval stage (81.4 for WT and 20.0 and 18.7 P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA, Figure 4A). This resulted in a significant reduction in the percentage of worms reaching the adulthood, being the 88.6 for WT nematodes and 13.8 and 22.9 for P32G and DN6 transgenic animals, respectively (p,0.01vs. WT, One-way ANOVA) and indicates that the expression of the mutated or truncated isoforms of the protein affected the nematodes growth and development. The phenotypic abnormality well correlated with the aggregation pathway of b2-m. In particular, a correlation coefficient ofR = 0.979 was determined when the percentage of transgenic worms reaching the adulthood, 72 hours after synchronization, was plotted with the amount of A11-positive oligomeric assemblies detected by dot blotting (Figure 4B). To determine whether b2-m affected the health of nematodes and their lifespan, the overall nematodes survival was evaluated. The expression of wild type b2-m significantly decreased the median lifespan of transgenic worms compared to nematodes injected with the empty vector (Figure 4C, median survival respectively: 13 days and 10 days for Vector and WT, p,0.05, Wilcoxon test). The insertion of both the P32G mutated gene and deleted DN6 sequence similarly shortened the survival of worms by 38 compared to the empty vector (median of survival: 8 days for both P32G and DN6, p,0.001 vs. Vector, Wilcoxon test) and by 20 compared to WT (p,0.01, Wilcoxon test). Thus, nematodes expressing the mutated or truncated gene had a shorter lifespan, indicating that, in vivo, P32G and DN6 show a greater proteotoxicity than WT b2-m. The presence of misfolded proteins in body wall muscle cells can induce dysfunctions in the coordination and motility of C. elegans [6].C. elegans Models for b2-m AmyloidosisFigure 3. Localization of b2-m in transgenic C. elegans strains. Overlay of bright field and immunofluorescence images of head, vulva and tail of transgenic C. elegans strains. All animals depicted are 2 days adult worms. A specific b2-m related signal (red, using a polyclonal anti human b2-m antibody) was observed at the vulva muscles and anal sphincter muscle in the tail (red arrows) whereas no signal was observed in the head muscles. Scale bar, 50 mm. doi:10.1371/journal.pone.0052314.gWe investigated whether.H lane and immunoblotted with polyclonal anti-human b2-m antibody (Dako). (D) Representative dot blot developed by antibody recognizing oligomers (A11) in transgenic worms and (E) quantification of A11-immunoreactive bands. Data are expressed as mean of density of A11 immunoreactive bands/mg of protein 6 SE of three independent experiments (N = 9); *p,0.01 vs WT, according to one-way ANOVA. doi:10.1371/journal.pone.0052314.gtherefore the growth rate is constant within larval phases and, reached a plateau in late adulthood [28]. After synchronization, the numbers of worms were scored after 24, 48 and 72 hours that correspond to the L1/L2, L2/L3 and L4/adult larval stages, respectively. WT nematodes exhibited a constant number of worms and a constant growth rate similarly to that observed in animals transfected with the empty vector (Figure 4A). In P32G and DN6 transgenic C. elegans strains, the percentage of worms reaching the L1/L2 stage was significantly reduced than in WT (83.3 for WT and 27.6 and 37.8 for P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA). The irregular growth rate compared to WT was also observed at the L2/L3 larval stage (81.4 for WT and 20.0 and 18.7 P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA, Figure 4A). This resulted in a significant reduction in the percentage of worms reaching the adulthood, being the 88.6 for WT nematodes and 13.8 and 22.9 for P32G and DN6 transgenic animals, respectively (p,0.01vs. WT, One-way ANOVA) and indicates that the expression of the mutated or truncated isoforms of the protein affected the nematodes growth and development. The phenotypic abnormality well correlated with the aggregation pathway of b2-m. In particular, a correlation coefficient ofR = 0.979 was determined when the percentage of transgenic worms reaching the adulthood, 72 hours after synchronization, was plotted with the amount of A11-positive oligomeric assemblies detected by dot blotting (Figure 4B). To determine whether b2-m affected the health of nematodes and their lifespan, the overall nematodes survival was evaluated. The expression of wild type b2-m significantly decreased the median lifespan of transgenic worms compared to nematodes injected with the empty vector (Figure 4C, median survival respectively: 13 days and 10 days for Vector and WT, p,0.05, Wilcoxon test). The insertion of both the P32G mutated gene and deleted DN6 sequence similarly shortened the survival of worms by 38 compared to the empty vector (median of survival: 8 days for both P32G and DN6, p,0.001 vs. Vector, Wilcoxon test) and by 20 compared to WT (p,0.01, Wilcoxon test). Thus, nematodes expressing the mutated or truncated gene had a shorter lifespan, indicating that, in vivo, P32G and DN6 show a greater proteotoxicity than WT b2-m. The presence of misfolded proteins in body wall muscle cells can induce dysfunctions in the coordination and motility of C. elegans [6].C. elegans Models for b2-m AmyloidosisFigure 3. Localization of b2-m in transgenic C. elegans strains. Overlay of bright field and immunofluorescence images of head, vulva and tail of transgenic C. elegans strains. All animals depicted are 2 days adult worms. A specific b2-m related signal (red, using a polyclonal anti human b2-m antibody) was observed at the vulva muscles and anal sphincter muscle in the tail (red arrows) whereas no signal was observed in the head muscles. Scale bar, 50 mm. doi:10.1371/journal.pone.0052314.gWe investigated whether.H lane and immunoblotted with polyclonal anti-human b2-m antibody (Dako). (D) Representative dot blot developed by antibody recognizing oligomers (A11) in transgenic worms and (E) quantification of A11-immunoreactive bands. Data are expressed as mean of density of A11 immunoreactive bands/mg of protein 6 SE of three independent experiments (N = 9); *p,0.01 vs WT, according to one-way ANOVA. doi:10.1371/journal.pone.0052314.gtherefore the growth rate is constant within larval phases and, reached a plateau in late adulthood [28]. After synchronization, the numbers of worms were scored after 24, 48 and 72 hours that correspond to the L1/L2, L2/L3 and L4/adult larval stages, respectively. WT nematodes exhibited a constant number of worms and a constant growth rate similarly to that observed in animals transfected with the empty vector (Figure 4A). In P32G and DN6 transgenic C. elegans strains, the percentage of worms reaching the L1/L2 stage was significantly reduced than in WT (83.3 for WT and 27.6 and 37.8 for P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA). The irregular growth rate compared to WT was also observed at the L2/L3 larval stage (81.4 for WT and 20.0 and 18.7 P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA, Figure 4A). This resulted in a significant reduction in the percentage of worms reaching the adulthood, being the 88.6 for WT nematodes and 13.8 and 22.9 for P32G and DN6 transgenic animals, respectively (p,0.01vs. WT, One-way ANOVA) and indicates that the expression of the mutated or truncated isoforms of the protein affected the nematodes growth and development. The phenotypic abnormality well correlated with the aggregation pathway of b2-m. In particular, a correlation coefficient ofR = 0.979 was determined when the percentage of transgenic worms reaching the adulthood, 72 hours after synchronization, was plotted with the amount of A11-positive oligomeric assemblies detected by dot blotting (Figure 4B). To determine whether b2-m affected the health of nematodes and their lifespan, the overall nematodes survival was evaluated. The expression of wild type b2-m significantly decreased the median lifespan of transgenic worms compared to nematodes injected with the empty vector (Figure 4C, median survival respectively: 13 days and 10 days for Vector and WT, p,0.05, Wilcoxon test). The insertion of both the P32G mutated gene and deleted DN6 sequence similarly shortened the survival of worms by 38 compared to the empty vector (median of survival: 8 days for both P32G and DN6, p,0.001 vs. Vector, Wilcoxon test) and by 20 compared to WT (p,0.01, Wilcoxon test). Thus, nematodes expressing the mutated or truncated gene had a shorter lifespan, indicating that, in vivo, P32G and DN6 show a greater proteotoxicity than WT b2-m. The presence of misfolded proteins in body wall muscle cells can induce dysfunctions in the coordination and motility of C. elegans [6].C. elegans Models for b2-m AmyloidosisFigure 3. Localization of b2-m in transgenic C. elegans strains. Overlay of bright field and immunofluorescence images of head, vulva and tail of transgenic C. elegans strains. All animals depicted are 2 days adult worms. A specific b2-m related signal (red, using a polyclonal anti human b2-m antibody) was observed at the vulva muscles and anal sphincter muscle in the tail (red arrows) whereas no signal was observed in the head muscles. Scale bar, 50 mm. doi:10.1371/journal.pone.0052314.gWe investigated whether.H lane and immunoblotted with polyclonal anti-human b2-m antibody (Dako). (D) Representative dot blot developed by antibody recognizing oligomers (A11) in transgenic worms and (E) quantification of A11-immunoreactive bands. Data are expressed as mean of density of A11 immunoreactive bands/mg of protein 6 SE of three independent experiments (N = 9); *p,0.01 vs WT, according to one-way ANOVA. doi:10.1371/journal.pone.0052314.gtherefore the growth rate is constant within larval phases and, reached a plateau in late adulthood [28]. After synchronization, the numbers of worms were scored after 24, 48 and 72 hours that correspond to the L1/L2, L2/L3 and L4/adult larval stages, respectively. WT nematodes exhibited a constant number of worms and a constant growth rate similarly to that observed in animals transfected with the empty vector (Figure 4A). In P32G and DN6 transgenic C. elegans strains, the percentage of worms reaching the L1/L2 stage was significantly reduced than in WT (83.3 for WT and 27.6 and 37.8 for P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA). The irregular growth rate compared to WT was also observed at the L2/L3 larval stage (81.4 for WT and 20.0 and 18.7 P32G and DN6, respectively, p,0.01 vs. WT, one-way ANOVA, Figure 4A). This resulted in a significant reduction in the percentage of worms reaching the adulthood, being the 88.6 for WT nematodes and 13.8 and 22.9 for P32G and DN6 transgenic animals, respectively (p,0.01vs. WT, One-way ANOVA) and indicates that the expression of the mutated or truncated isoforms of the protein affected the nematodes growth and development. The phenotypic abnormality well correlated with the aggregation pathway of b2-m. In particular, a correlation coefficient ofR = 0.979 was determined when the percentage of transgenic worms reaching the adulthood, 72 hours after synchronization, was plotted with the amount of A11-positive oligomeric assemblies detected by dot blotting (Figure 4B). To determine whether b2-m affected the health of nematodes and their lifespan, the overall nematodes survival was evaluated. The expression of wild type b2-m significantly decreased the median lifespan of transgenic worms compared to nematodes injected with the empty vector (Figure 4C, median survival respectively: 13 days and 10 days for Vector and WT, p,0.05, Wilcoxon test). The insertion of both the P32G mutated gene and deleted DN6 sequence similarly shortened the survival of worms by 38 compared to the empty vector (median of survival: 8 days for both P32G and DN6, p,0.001 vs. Vector, Wilcoxon test) and by 20 compared to WT (p,0.01, Wilcoxon test). Thus, nematodes expressing the mutated or truncated gene had a shorter lifespan, indicating that, in vivo, P32G and DN6 show a greater proteotoxicity than WT b2-m. The presence of misfolded proteins in body wall muscle cells can induce dysfunctions in the coordination and motility of C. elegans [6].C. elegans Models for b2-m AmyloidosisFigure 3. Localization of b2-m in transgenic C. elegans strains. Overlay of bright field and immunofluorescence images of head, vulva and tail of transgenic C. elegans strains. All animals depicted are 2 days adult worms. A specific b2-m related signal (red, using a polyclonal anti human b2-m antibody) was observed at the vulva muscles and anal sphincter muscle in the tail (red arrows) whereas no signal was observed in the head muscles. Scale bar, 50 mm. doi:10.1371/journal.pone.0052314.gWe investigated whether.