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The value of polymerase chain reaction detection of Mycobacterium tuberculosis in granulomas isolated by laser capture microdissection
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The value of polymerase chain reaction detection of Mycobacterium tuberculosis in granulomas isolated by laser capture microdissection ERIC SELVA*, VERONIQUE HOFMAN*$, FREDERICK BERTO*, SANDRA MUSSO$, LAURENT CASTILLO%, JOSE SANTINI%, PIERRE DELLAMONICA# AND PAUL HOFMAN* $ *INSERM 02-15, IFR 50, $Department of Pathology, %Department of Otorhinolaryngology, and #Department of Infectious Disease, University of Nice, Nice, France Pathology(February 2004)36(1), pp. 77-81
Introduction Mycobacterium tuberculosis in 2004 High infection Drug resistant Methods for detecting mycobacteria Cultural identification Ziehl-Neelsen(ZN)stain PCR Ile de France Provence Alpes Côte d’Azur
Introduction Cultural identification Standard method Antibiotic sensitivity Fresh specimen Take up to 6 weeks Ziehl-Neelsen(ZN)stain Acid-fast bacilli Not sensitive Not identification species
Introduction Polymerase chain reaction(PCR) Perform rapidly High sensitivity High specificity >20μm in thickness False positive False negative
Introduction LCM ┼ PCR on FFPE Increase efficiency Overcome problem FFPE Formalin fixed paraffin embedded
Materials Lymph nodes from 49 case of inflammatory necrotizing granuloma Department of pathology of Pasteur Hospital, University of Nice, France 1990 – 1998
Methods Laser capture microdissection 5μm tissue section Deparaffinised and H&E stain Microdissect using LCM microscope(PixCell Ⅱ, Arcturus Engineering, Alphelys, Paris, France) DNA extraction Clean with xylene
Methods Whole section DNA extraction(1) 10 whole cross 5μm tissue sections Deparaffinised by 1mL xylene, 20 minutes, 65℃, then 14000 rpm, 2 minutes, remove supernatant, twice Washing 1mL 100%ethanol, 5 minutes, then 14000 rpm, 5 minutes, twice Dried in a speed vacuum
Methods Whole section DNA extraction(2) Digestion buffer: Distilled water Proteinase K;100 μg/ μl;Sigma, Paris Tris HCl;20mM;pH8.0 EDTA;20mM;Sigma SDS;2% Digestion 72 hours, 55℃
Methods Whole section DNA extraction(3) 14000 rpm, 5 minutes The supernatant = template for PCR DNA concentration and purity: Absorbency at 260 and 280 λ(Ultraspec 2000, USA)
Methods PCR(1) 1μl DNA template;50mM KCl;10mM Tris HCl, pH8.3;dH2O;1.5mM MgCl2;dNTPs(200μM;Invitrogen, Paris, France);primer 1;primer 2;Taq Polymerase(1.25U; Invitrogen);final 50 μl
Methods PCR(2) Sequence of primer : Primer 1(IS6110 5’): 5’– 3’:CCTGCGAGCGTAGGCGTCGG Primer 2(IS6110 3’): 5’– 3’:CTCGTCCAGCGCCGCTTCGG 16S ribosomal RNA gene of M. tuberculosis
Methods PCR(3) Condition for PCR : 94℃ 5 minutes 67℃ 1 minutes 72℃ 40 seconds 35 cycles Perkin – Elmer Thermal Cycler;CA, USA
Methods Electrophoresis 8μl PCR product 2μl bromophenol blue(Ficoll) 1.5% agarose, ethidium bromide – stained gel 135 V 30 minutes
Methods DNA isolation control: Amplification of β-actin gene β-actin 5’:3’– AGCGGGAAATCGTGCGTG β-actin 3’:5’– CAGGGTACATGGTGGTGC Invitrogen, Paris, France
Methods PCR control: 5 cases of sarcoidosis 5 cases of lymph nodes from HIV patients who presented with atypical mycobacteriosis(with positive culture for M. avium intracellulare) Paraffin block without tissue
Results PCR from microdissected granulomas and correlation with PCR from whole sections(1)
Results PCR from microdissected granulomas and correlation with PCR from whole sections (2) ※4 cases were negative both ※The signal obtained from microdissected granulomas was weaker than the signal obtained from whole sections ※All negative controls were negative both ※The latter case had been embedded more than 8 years
Results Correlation of PCR from microdissected granulomas with acid fast stained tissue
Results Correlation of PCR from microdissected granulomas with culture
Discussion ※Infectious diseases => Granulomas ※Detection of granuloma => Diagnosis of Tuberculosis ※Determination the causative agent => Special stain *Sensitivity *Specificity
Discussion ※Cultural identification: *Mycobacterial infection may not have been clinically suspected and specimens not obtained for culture. ※Molecular diagnosis of M. tuberculosis =>PCR(whole section) ※ PCR positive rate=>DNA quantity ※ PCR false negative=>2%~19% (whole section)
Discussion ※The PCR performed from whole sections may present some disadvantages: *An excessive material-consuming method on small specimens. *Increasing the effect of tissue inhibitors or contamination. ※Lesion <=> PCR result *Relatively low amount of specimen *PCR-based analysis for amplification
Discussion ※LCM:
Discussion ※PCR detection of M. tuberculosis: *Sensitivity=>92% *Specificity=>100% ※LCM +PCR : *Useful on small specimen *Reduce false positive due to contamination ※Successful confirmation of M. tuberculosis * (×) Tissue DNA * (o) Digestion for obtain M. tuberculosis DNA
Discussion IS6110 : CCT GCG AGC GTA GGC GTC GG CTC GTC CAG CGC CGC TTC GG TB11/12: ACC AAC GAT GGT GTG TCC AT CTT GTC GAA CCG CAT ACC CT TB2A/2B: GAG ATC GAG GTC GAG GAT CC AGC TGC AGC CCA AAG GTG TT