He preceding 4 weeks, were recruited as cases if their parents-guardians gave written informed consent. Haemoglobin CI-1011 site concentration was measured at the time of recruitment by the HemoCueH system (HemoCueH HB 201+, ?Anghelom, Sweden). A complete clinical examination was performed and the information was entered onto standardized questionnaires together with demographic data. Four ml of venous blood were collected by venipuncture for K162 chemical information malaria parasitaemia examination, bacterial culture, full blood count and biochemical and molecular determinations. Participating children were offered voluntary HIV counselling and testing. A bone marrow aspiration was performed from the anterior-superior iliac crest or the tibia, under conscious sedation with parenteral ketamine, atropine and diazepam [29,30,31]. Bone marrow aspirates were not performed in children ,3 months of age or with medical counter-indications such as severe respiratory distress, history of seizures, suspected intracranial hypertension, or any risk at the discretion of the responsible clinician. There were no adverse effects associated to bone marrow biopsy, however there were three adverse effects associated to sedation. One child presented bronchial hypersecretion and bone marrow aspirate was then not performed. Two other children vomited during the aspirate, also due to the administration of sedatives. Resuscitation equipment was always available during the procedure. All children received treatment according to their clinical condition and following national guidelines.Laboratory MethodsA complete blood count was performed on an automated haematology analyzer Sysmex XT-2000i (Sysmex Corporation, Randburg, South Africa). P. falciparum parasites were identified by microscopy of thick and thin Giemsa-stained blood films [32]. P. falciparum-specific real time quantitative PCR (qPCR) was performed on microscopically negative samples [33]. HIV status was assessed using the Determine HIV-1/2 Rapid Test (Abbott Laboratories, Abbott Park, IL) and positive results were confirmed by the Uni-Gold Rapid Test (Trinity Biotech Co., Wicklow, Ireland). For children ,18 months who were positive by both HIV rapid tests and for cases with discordant results, HIV infection was confirmed using the HIV-1 DNA-PCR kit (Roche MolecularStudy Participants and ProceduresThe study was undertaken as part of a case-control study on the aetiology and risk factors of anaemia in 18325633 children less than 5 years of age. Children aged 1 to 59 months, attending the MDH emergency department between October 2008 to AugustIron Deficiency Diagnosis and InfectionsFigure 1. Receiver operating characteristic curves of the iron markers in the identification of iron stores deficiency. Cut-off values for sTfR and TfR-F index with the highest sensitivity to detect iron deficiency maintaining the specificity 50 are indicated with arrows. Abbreviations: Sat. Transf., transferrin saturation; sTfR, soluble transferrin receptor; TfR-F index, transferrin-ferritin index; TIBC, total iron binding capacity. doi:10.1371/journal.pone.0050584.gSystems, Branchburg, NJ, USA) [34,35]. Blood was cultured using an automated system (BACTECH 9050; Becton-Dickinson, Franklin Lake, NJ, USA) [36,37]. Epstein-Barr virus (EBV) and Parvovirus B19 (PV-B19) were identified by real time qPCR using the Artus EBV RG PCR and the Artus Parvo B19 RG PCR kits (QIAGEN), respectively. Diagnosis of a-thalassaemia (3.7 kb deletion) was performed by the GAP-PCR [38] in 121.He preceding 4 weeks, were recruited as cases if their parents-guardians gave written informed consent. Haemoglobin concentration was measured at the time of recruitment by the HemoCueH system (HemoCueH HB 201+, ?Anghelom, Sweden). A complete clinical examination was performed and the information was entered onto standardized questionnaires together with demographic data. Four ml of venous blood were collected by venipuncture for malaria parasitaemia examination, bacterial culture, full blood count and biochemical and molecular determinations. Participating children were offered voluntary HIV counselling and testing. A bone marrow aspiration was performed from the anterior-superior iliac crest or the tibia, under conscious sedation with parenteral ketamine, atropine and diazepam [29,30,31]. Bone marrow aspirates were not performed in children ,3 months of age or with medical counter-indications such as severe respiratory distress, history of seizures, suspected intracranial hypertension, or any risk at the discretion of the responsible clinician. There were no adverse effects associated to bone marrow biopsy, however there were three adverse effects associated to sedation. One child presented bronchial hypersecretion and bone marrow aspirate was then not performed. Two other children vomited during the aspirate, also due to the administration of sedatives. Resuscitation equipment was always available during the procedure. All children received treatment according to their clinical condition and following national guidelines.Laboratory MethodsA complete blood count was performed on an automated haematology analyzer Sysmex XT-2000i (Sysmex Corporation, Randburg, South Africa). P. falciparum parasites were identified by microscopy of thick and thin Giemsa-stained blood films [32]. P. falciparum-specific real time quantitative PCR (qPCR) was performed on microscopically negative samples [33]. HIV status was assessed using the Determine HIV-1/2 Rapid Test (Abbott Laboratories, Abbott Park, IL) and positive results were confirmed by the Uni-Gold Rapid Test (Trinity Biotech Co., Wicklow, Ireland). For children ,18 months who were positive by both HIV rapid tests and for cases with discordant results, HIV infection was confirmed using the HIV-1 DNA-PCR kit (Roche MolecularStudy Participants and ProceduresThe study was undertaken as part of a case-control study on the aetiology and risk factors of anaemia in 18325633 children less than 5 years of age. Children aged 1 to 59 months, attending the MDH emergency department between October 2008 to AugustIron Deficiency Diagnosis and InfectionsFigure 1. Receiver operating characteristic curves of the iron markers in the identification of iron stores deficiency. Cut-off values for sTfR and TfR-F index with the highest sensitivity to detect iron deficiency maintaining the specificity 50 are indicated with arrows. Abbreviations: Sat. Transf., transferrin saturation; sTfR, soluble transferrin receptor; TfR-F index, transferrin-ferritin index; TIBC, total iron binding capacity. doi:10.1371/journal.pone.0050584.gSystems, Branchburg, NJ, USA) [34,35]. Blood was cultured using an automated system (BACTECH 9050; Becton-Dickinson, Franklin Lake, NJ, USA) [36,37]. Epstein-Barr virus (EBV) and Parvovirus B19 (PV-B19) were identified by real time qPCR using the Artus EBV RG PCR and the Artus Parvo B19 RG PCR kits (QIAGEN), respectively. Diagnosis of a-thalassaemia (3.7 kb deletion) was performed by the GAP-PCR [38] in 121.