Reticulated platelets as a screening test to identify thrombocytopenia aetiology

doi:10.1093/qjmed/hcn047

QJM Advance Access originally published online on April 8, 2008
QJM 2008 101(7):549-555; doi:10.1093/qjmed/hcn047

This Article

	Full Text
	FREE Full Text (PDF)
	All Versions of this Article: 101/7/549 most recent hcn047v1
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Email this article to a friend
	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Add to My Personal Archive
	Download to citation manager
	Search for citing articles in: ISI Web of Science (5)
	Request Permissions
	Disclaimer

Google Scholar

	Articles by Monteagudo, M.
	Articles by Tolosa, C.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Monteagudo, M.
	Articles by Tolosa, C.

Social Bookmarking

	What's this?

Reticulated platelets as a screening test to identify thrombocytopenia aetiology

M. Monteagudo¹, Ma J. Amengual², L. Muñoz³, J.A. Soler³, I. Roig³ and C. Tolosa¹

From the ¹Internal Medicine Department, ²Immunology Laboratory, and ³Hematology Service, Hospital de Sabadell, Institut Universitari Parc Tauli—UAB, Sabadell, Barcelona, Spain

Address correspondence to M. Monteagudo, Internal Medicine Department, Hospital de Sabadell, Parc Taulí S/N, 08208 Sabadell, Barcelona, Spain. email: MMonteagudo{at}tauli.cat

Received 9 October 2007 and in revised form 11 March 2008

Abstract

Background: Thrombocytopenia is a common haematological abnormalityand no simple diagnostic test is available to diagnose thrombocytopeniapathogenesis.

Aim: To evaluate sensitivity and specificity of reticulatedplatelets (RP) as a diagnostic test for thrombocytopenia withincreased thrombopoietic activity.

Design: Prospective observational study in thrombocytopenicpatients.

Methods: A direct, whole-blood, dual-labelling flow cytometricmethod was used. Direct, whole-blood double coverage was achievedusing a monoclonal anti-glycoprotein (GP)-III antibody (CD61PerCP®) for platelet identification and thiazole orange(Retic-count®) as platelet mARN stain.

Results: RP were measured in 101 thrombocytopenic patients and104 non-thrombocytopenic controls. The mean RP percentage in60 thrombocytopenic patients with no increased thrombopoieticactivity was 7.5% (CI for 95%: 5.2–9.7) and RP absolutenumber was 3.2 x 10⁹/l (CI for 95%: 2.1–4.3). The meanRP percentage in 41 thrombocytopenic patients with increasedthrombopoietic activity was 30.3% (CI for 95%: 25.1–35.5)and RP absolute number was 6.2 (CI for 95%: 4.8–7.7).The RP percentage cut-off for a diagnosis of thrombocytopeniawith increased thrombopoietic activity was 11% [sensitivity93%, specificity 85%, positive predictive value (PPV) 83%, negativepredictive value (NPV) 95%].

Conclusions: RP measurement by flow cytometry, directly fromwhole-blood, is a useful screening test to differentiate betweenthrombocytopenia with high or low thrombopoietic activity. ARP percentage in excess of 11%, has a high sensitivity and goodspecificity for a diagnosis of thrombocytopenia with increasedthrombopoietic activity.

Add to CiteULike CiteULike Add to Connotea Connotea Add to Del.icio.us Del.icio.us What's this?