Kevin J. Trainor scite author profile

The polymerase chain reaction (PCR) was used to develop a simple technique for detecting monoclonality at the DNA level in B lymphocyte populations in formalin fixed, paraffin wax embedded material. Sections were dewaxed and dehydrated, and the DNA was extracted by boiling in water for 45 minutes. A semi-nested PCR was performed to amplify the V-D-J region of the immunoglobulin heavy chain gene. The product was electrophoresed and viewed under ultraviolet light after ethidium bromide staining. Specimens from 26 B cell lymphomas produced a monoclonal band in 24 cases and no amplification in two cases; monoclonality was specific for this disorder. Specimens from seven T cell lymphomas produced no amplification; specimens from nine reactive nodes produced a broad smear of polyclonal material; and specimens from 12 cases of carcinoma produced either no amplification or polyclonal material.As detection of monoclonality is strongly suggestive of neoplastic disease, this technique is likely to be of value in routine diagnosis, because of its speed, simplicity, and applicability to fixed, embedded material.

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Integrating information technology and marketing: An examination of the drivers and outcomes of e-Marketing capability

Trainor

Rapp

Beitelspacher

et al. 2011

Industrial Marketing Management

174

121

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Kevin J. Trainor

Social media technology usage and customer relationship performance: A capabilities-based examination of social CRM

Performance implications of customer-linking capabilities: Examining the complementary role of customer orientation and CRM technology

Relating Social Media Technologies to Performance: A Capabilities-Based Perspective

Monoclonality in B cell lymphoma detected in paraffin wax embedded sections using the polymerase chain reaction.

Integrating information technology and marketing: An examination of the drivers and outcomes of e-Marketing capability

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