Modification of IgH PCR clonal analysis by the addition of sucrose and cresol red directly to PCR reaction mixes.
Open Access
- 1 June 1997
- journal article
- Published by BMJ in Molecular Pathology
- Vol. 50 (3) , 164-166
- https://doi.org/10.1136/mp.50.3.164
Abstract
Diagnostic immunoglobulin (Ig) polymerase chain reaction (PCR) clonality analyses need to be simple, reproducible, and rapid. Sucrose and cresol red (gel loading buffer reagents) were added to a routine IgH PCR reaction mix to obviate the need for adding gel loading buffer separately after PCR amplification. Not only did this decrease the time spent after PCR analysis but also gave similar or enhanced IgH PCR product intensity compared with normal IgH PCR conditions on polyacrylamide gel electrophoresis. This procedure was easily adapted to routine PCR analysis without the need for further manipulations or optimisation of the PCR reaction mix, and it increased the reproducibility and specificity of the IgH PCR products.Keywords
This publication has 8 references indexed in Scilit:
- Investigation of specimen mislabelling in paraffin‐embedded tissue using a rapid, allele‐specific, PCR‐based HLA class II typing methodHistopathology, 1996
- Expanded TcR V beta 5.1 family in a diffuse high-grade B cell immunoblastic lymphoma.1995
- Enhancement of HLA class II PCR-SSP typing by addition of cresol red and sucrose to the amplification mixturesHuman Immunology, 1994
- Sources of DNA for detecting B cell monoclonality using PCR.Journal of Clinical Pathology, 1994
- Gel-loading dyes compatible with PCR.1992
- Detection of clonality in childhood B-lineage acute lymphoblastic leukaemia by the polymerase chain reaction.1992
- PCR Amplification from Paraffin-Embedded Tissues: Effects of Fixative and Fixation TimeAmerican Journal of Clinical Pathology, 1991
- Tissue extraction of DNA and RNA and analysis by the polymerase chain reaction.Journal of Clinical Pathology, 1990