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Assessment of monoclonality in large B cell non-Hodgkins lymphoma

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Presentation on theme: "Assessment of monoclonality in large B cell non-Hodgkins lymphoma"— Presentation transcript:

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2 Assessment of monoclonality in large B cell non-Hodgkins lymphoma
Lotfi N. M.Sc Rastin M, Ph.D Memar B, MD Mahmoudi M. MD, Ph.D Immunology Research Center, BuAli Research Institute, Mashhad University of Medical Sciences

3 Introduction

4 Subdivision of large B-cell lymphomas by morphology
Diffuse large B-cell lymphoma (DLBCL) 40% of adult Non-Hodgkin lymphomas - Morphologically, genetically and clinically heterogeneous group of large B cells tumors Subdivision of large B-cell lymphomas by morphology Centroblastic lymphoma Immunoblastic lymphomas

5 Composed of large cells Resemble centroblasts or immunoblasts
Often with a mixture of the two Clinical significance is yet debated Centroblastic type (80% of the cases) is composed of : - cells resembling germinal center centroblasts - with one to three peripheral nucleoli - a narrow rim of basophilic cytoplasm -mixture of both immunoblasts and centroblasts

6 In crucial cases: Morphological criteria do not help distinguish
Diagnosis of NHL still represents a challenge In reactive and malignant lymphoproliferations Molecular Diagnostic methods are useful tools Clonality assays are helpful

7 Demonstration of monoclonality in gene level
In B cell lymphomas is of great importance Distinguish lymphomas from reactive lymphoid lesions When morphological and immunophenotypic features are difficult to interpret

8 Southern blot analysis of Ig genes:
Is the established method for monoclonality demonstration However it is: Slow Complex Requires fresh samples Expensive

9 Detection of B cell monoclonoclonality
PCR Polymerase chain reaction overcome limitations - Offers : Sensitive Rapid Simple Flexible Detection of B cell monoclonoclonality

10 PCR approach based on : -Amplification of VDJ region of rearranged Ig heavy chain gene in lymphoid tissues - Followed by size analysis of products On an electrophoretic gel.

11 DH VH JH CH 5´ 3´ DH-N-JH VH-N-DH-N-JH CDR3 5´ FR1 FR2 FR3 N D N FR4
bp

12 Methods & Materials

13 Receiving sample blocks from Pathology archive
Reading OD and PCR with beta actin primer Receiving sample blocks from Pathology archive Electrophoresis and staining Method DNA Extraction PCR with Specific primers 13

14 Samples obtained from:
archives of : Imam Reza Ghaem Omid Hospitals private laboratories in Mashhad Samples include 44 DLBCL specimens 20 samples from tonsil and appendix as controls These cases were reviewed by a pathologist for confirmation.

15 5 µm sections were cut from paraffin blocks
Samples were deparraffinized DNA extracted using proteinase K digestion method

16 Amplification of house keeping gene
ß -Actin gene amplified To confirm extracted DNA quality

17 PCR reaction

18 Electrophoresis and staining
To analyze the PCR products : 15µl of each PCR product was electrophoresed on 8% PAGE Stained with AgNo3

19 Results

20 MW 50 bp FR3 N D JH ‍JH

21 FR3 N D ‍JH 50 bp MW

22 100 bp (c) MW 125bp

23 Results: - all samples had adequate DNA quality
- using primers amplifyng FRIII-JH region - clonal IgH gene rearrangements - demonstrated in 75%(33/44) of the cases. Monoclonality Positive Results Number Samples %75 33 44 DLBCL %0 20 Control

24 Disccusion and conclusion

25 1993 Fc- Linng et al 2002 Yon- Chin- Tai et al Adan-Begg et al 2003
Results Year Previous studies 56% 1993 Fc- Linng et al 54.3% 2002 Yon- Chin- Tai et al 47% Adan-Begg et al 55% 2003 Timeap. Gurbitty et al

26 - Previoue Studies on Diffuse large B cell lymphomas - Reported 47%-55% with the FR3/JH - we succeed to increase the diagnosis to 75% - using new design of primers (degenarate primers)

27 PCR method is: - Sensitive & Reliable - for detecting B cell clonality Can be used as an accessory diagnostic tool to conventional assessment of lymphoprolyferative diseases.

28 Thanks for Your Attention

29 Thanks for Your Attention

30 100 bp

31 M M

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