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Real-Time PCR Applications: • Detection of chromosomally mediated penicillin-resistant Neisseria gonorrhoeae • Quantitative expression of mRNA encoding pro-inflammatory and immunomodulatory cytokines in hamsters infected with a virulent variant of Leptospira IPNC Juillet 2006 1 Neisseria gonorrhoeae the etiologic agent for the sexually transmitted infection gonorrhoea 2 • Second most common bacterial STD in France as in US • Around 75% of all reported cases in 15-29 year old age group • High prevalences reported from non-genital sites among MSM (oropharynx & rectum) • Usually symptomatic in males, often asymptomatic in women • Can cause PID, infertility, ectopic pregnancy, and complications in pregnancy in women Présentation des activités de l’Institut Pasteur Treatment Depending of the national guidelines • 1940s = Penicillin effective treatment • 1970s = Penicillin resistance develops secondary to acquisition of plasmid for penicillinase • Since 1972, CDC has recommended treatment with third generation cephalosporin or fluoroquinolones (SD) • Increase in chromosomally acquired multi-resistance to antibiotics • In New Caledonia, N.gonorrhoeae were susceptible to penicillin • 3 Benzylpenicillin, metronidazole and azithromycin Présentation des activités de l’Institut Pasteur Mechanisms of antibiotic resistance • Alteration of the target site • Reduction of the affinity for the antibiotic • Access of the antibiotic to the target site • Reduced permeability of the cell envelope • Active export of antibiotics • Destruction of the antibiotic 4 Présentation des activités de l’Institut Pasteur b-lactams action mode Antibiotics Penicillin binding proteins 5 Présentation des activités de l’Institut Pasteur Mechanisms of penicillin resistance in N. Gonorrhoeae (1) Plasmid mediated b-lactamases Acquired, Transferable (e.g. TEM) Chromosomally- mediated alterations • Altered penicillin binding proteins • Porins • Efflux pumps is of considerable concern 6 Présentation des activités de l’Institut Pasteur Mechanisms of penicillin resistance in N.gonorrhoeae (2) 7 Présentation des activités de l’Institut Pasteur Real-Time Multiplex PCR Assay • Detection of NG from clinical samples within 2hrs • Combined detection of penA and ponA genotypes • ponA mutation = T to C substitution (CMI ≥ 1 mg/ml) • penA mutation = additional aspartic acid (Asp-345A) codon (CMI ≥ 0.03 mg/ml) • Correlation with Phenotypes obtained by E-test • Status of N.gonorrhoeae strains in New Caledonia • LightCycler: additional advantage 8 Présentation des activités de l’Institut Pasteur Oligonucleotide sequences Design with Probe design software 2.0 (Roche Diagnostics) Oligonucleotides ponA Primers ponA-F (Forward) ponA-R (Reverse) Probes ponA-P1 (Anchor) Sequences (5’ to 3’) Concentrations ponA-P2 (Sensor) 0,5 M 1 M 0,2 M a Positions CGGGAACTGTATGAGAAAT GTCTCGCCCGTACCTA 814-832 1694-1679 GGCGTTGGGCGGTGGT-fluorescein 1232-1247 b 0,2 M LC-R705 -AAGAGCCGTTGCTGCA-phosphate 1250-1265 0,5 M GACCTTGGCCTATGAAGAG GGTTACGGAAACCATCAGATT 756-774 1461-1441 CGCGACGATACCCATGTTTACC-fluorescein LC-R640c-TCTTTGGATGTGCGCGGCATTATGCA-phosphate 1057-1078 1081-1106 penA Primers penA-F (Forward) penA-R (Reverse) Probes penA-P1 (Sensor) penA-P2 (Anchor) a 9 GenBank accession number; 1 M 0,2 M 0,2 M b LC-R705, LightCycler red 705; c LC-R640, LightCycler red 640 Présentation des activités de l’Institut Pasteur FRET based-system for the detection of ponA mutation (1) T 881 bp 3’ ponA-F 5’ 814 C or ponA-P1 FL LC705 GGCGTTGGGCGGTGGT 1232 D 5’ ponA-P2 3’ AAGAGCCGTTGCTGCA(PO4) A 1265 hυ ponA-R FRET 5’ 1679 5’ Forward Primer 10 3’ Anchor Probe Sensor Probe or Detection Probe Présentation des activités de l’Institut Pasteur Reverse Primer Tm and mutation detection 11 Présentation des activités de l’Institut Pasteur Overlap of emission spectra from fluorescent dyes used in the LC System • The degree of crosstalk is strongly influenced by: 12 • Temperature • Coupling chemistry of the fluorescence dyes • properties of the optical system Présentation des activités de l’Institut Pasteur Color compensation activation Without compensation With compensation 13 Présentation des activités de l’Institut Pasteur Experimental protocol (1) • Chromosomal DNA Extraction Using QIA amp DNA Minikit with : Isolated culture Urethral or vaginal samples (stocked in transport medium) Urines (resuspended in water after centrifugation) • Components of PCR with LightCycler FastStart DNA Master Hybridization Probes Kit (Roche ) Amorce penA-F (10 µM) Amorce penA-R (10 µM) Amorce ponA-F (10 µM) Amorce ponA-R (10 µM) Sonde penA-P1 (10 µM) Sonde penA-P2 (10 µM) Sonde ponA-P1 (10 µM) Sonde ponA-P2 (10 µM) Master mix 10X MgCl2 eau pcr 14 1 tube (µl) 1 2 1 2 0,4 0,4 0,4 0,4 2 2,4 6 18 µl mix et 2 µl ADN extrait Présentation des activités de l’Institut Pasteur Final 0,5 µM 1 µM 0,5 µM 1 µM 0,2 µM 0,2 µM 0,2 µM 0,2 µM 1X 4 mM Experimental protocol (2) 15 Présentation des activités de l’Institut Pasteur Partial sequence alignment 16 ponAWT 066213 275183 GTT CAA GAG CCG TTG CTG CAG GGG GCT TTG GTT TCG GTT CAA GAG CCG TTG CTG CAG GGG GCT TTG GTT TCG GTT CAA GAG CCG TTG CTG CAG GGG GCT TTG GTT TCG V Q E P L A L V S L Q G ponAmUT 356390 GTT CAA GAG CCG TTG CCG CAG GGG GCT TTG GTT TCG GTT CAA GAG CCG TTG CCG CAG GGG GCT TTG GTT TCG V Q E P L Q G A L V S P penAWT 037350 CCG TCT CCC GTG CGC … GAT ACC CAT GTT TAC CCC CCG TCT CCC GTG CGC … GAT ACC CAT GTT TAC CCC P S P V R D T H V Y P penAmUT 066213 CCG TCT CCC GTG CGC GAC GAT ACC CAT GTT TAC CCC CCG TCT CCC GTG CGC GAC GAT ACC CAT GTT TAC CCC P S P V R D T H V Y P D Présentation des activités de l’Institut Pasteur Characteristics of N. gonorrhoeae strains used in the study 38 MIC of Penicillin (g/ml) 0.016 et inf 9 0.032 S Asp-345A: 3/9 ponA mutant: 0/8 12 0.047 S Asp-345A: 9/12 ponA mutant: 0/12 8 0.064 I Asp-345A: 3/8 ponA mutant: 1/8 7 0.094 I Asp-345A: 7/7 ponA mutant: 0/6 3 0.19 I Asp-345A: 3/3 ponA mutant: 1/3 8 0.125 I Asp-345A: 8/8 ponA mutant: 1/8 6 0.25 I Asp-345A: 6/6 ponA mutant: 2/6 7 0.38 I Asp-345A: 6/7 ponA mutant: 4/7 2 0.5 I Asp-345A: 2/2 ponA mutant: 0/2 2 0.75 I Asp-345A: 2/2 ponA mutant: 2/2 18 1 et sup R Asp-345A: 18/18 ponA mutant: 18/18 Number of strains Phenotypic status penA genotype ponA genotype S Asp-345A: 2/38 ponA mutant: 0/38 120 NG strains 17 Présentation des activités de l’Institut Pasteur Gene expression at mRNA level Quantitative expression of mRNA encoding pro-inflammatory and immunomodulatory cytokines in hamsters infected with a virulent variant of Leptospira 18 Présentation des activités de l’Institut Pasteur Cytokines and immunity • Regulatory proteins • Inflammatory responses (TNFa vs IL-10) • Immune and pathological pathways Why quantifying cytokine expression? 19 • Specific immune mechanisms • Mechanisms of anti-Leptospira immunity • Th1-Th2 profile • Pathogenesis of infection Présentation des activités de l’Institut Pasteur Syrian hamster (Mesocricetus auratus) • Experimental model • Highly susceptible to Leptospira • Nucleotide sequence of cytokine genes (Melby et al., 1998) Quantification of specific cDNA targets • Absolute quantification • Relative quantification 20 Présentation des activités de l’Institut Pasteur Definition of used terms Definitions of Frequently Used Terms Term Definition Sample Material of interest (tissue, cells, blood etc.) Target Nucleic acid of interest (specific RNA or DNA sequence) Reference Nucleic acid that is found at a constant copy number in all samples (= endogenous control) The reference is used for normalization of sampleto-sample differences (nucleic acid quality and quantity). Housekeeping gene For mRNA quantification in gene expression studies. A gene that is expressed constitutively on an identical level in all samples to be analyzed. Calibrator 21 A sample that is used for normalization of the final results. The calibrator is positive for target and reference, and must have a constant expression ratio of target to reference. Présentation des activités de l’Institut Pasteur Absolute quantification 22 Présentation des activités de l’Institut Pasteur Relative quantification 23 Présentation des activités de l’Institut Pasteur Normalization Concentration of target Calibrator = Normalized Ratio Concentration of reference Concentration of target Concentration of reference 24 Présentation des activités de l’Institut Pasteur (sample) (calibrator) Standard Curve Generated with serial dilutions of a standard 25 Présentation des activités de l’Institut Pasteur From blood to curves 26 • 1 to 2 ml of blood • PBMC purification and in vitro culture • Stimulation of PBMC (LPS, PMA-ionomycin) • Total RNA extraction (High Pure RNA isolation kit, ROCHE) • cDNA preparation (Transcriptor First Strand cDNA synthesis kit, ROCHE) • LightCycler protocol (FastStart SYBR Green) • Specificity : melting curves, gel electrophoresis • cDNA dilutions (2 to 4x107 copies/µl) • Standard curves Présentation des activités de l’Institut Pasteur Standard curves E= 1,903 E= 1,899 E= 1,891 Ainsi que IL-1, IL-2, IL-4, IL-6, IL-10, IL-12p40 27 Présentation des activités de l’Institut Pasteur Set of target and reference genes 28 Cytokine Size Hyb. Temp. Tm IL-2 349 bp 61°C 85.2°C IL-4 342 bp 61°C 87.8°C IL-10 308 bp 61°C 87.8°C IL12p40 308 bp 61°C 89.9°C IFNg 226 bp 60°C 84.6°C TGFb 245 bp 60°C 90.0°C TNFa 278 bp 60°C 89.6°C HPRT 242 bp 60/61°C 82.4/82.9°C b actin 357 bp 60/61°C 90.0/90.4°C Présentation des activités de l’Institut Pasteur Expression profile of TNF-alpha 29 Présentation des activités de l’Institut Pasteur Expression profile of IFN-gamma 30 Présentation des activités de l’Institut Pasteur Ratio Expression profile of IL-12p40 2500 2000 1500 1000 500 0 1 31 2 4 6 8 10 18 22 D1 D2 D3 D4 Hours p.i. Days p.i. Présentation des activités de l’Institut Pasteur 4 2500 2000 3 +? 1500 2 1000 1 500 0 0 1 2 4 6 8 10 18 22 Hours p.i. 32 Présentation des activités de l’Institut Pasteur D1 D2 D3 Days p.i. D4 Ratio IL-12 Ratio IFN Expression profiles of g IFN and IL-12 From lymphocyte T to Th1 33 Présentation des activités de l’Institut Pasteur