Evaluation of erythropoiesis after bone marrow transplantation: quantitative reticulocyte counting

Davies, Sara; Cavill, I.; Bentley, Neil; Fegan, CD; Poynton, Christopher H.; Whittaker, J. A.

doi:10.1111/j.1365-2141.1992.tb08163.x

Cited by 54 publications

(32 citation statements)

References 6 publications

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“…These studies however, utilized different methods for measuring immature reticulocytes and/or compared the IRF to ANCX500/ml and not to the more clinically relevant ANCX100/ml (Table 4). 10,[15][16][17][18][19][20][21][22] Since there are different types and manufacturers of blood count analyzers with different reference values and calibration parameters, 9,23 end points such as doubling (IRF-D) or normalization (IRF-N) of the IRF can be used regardless of equipment and would simplify and standardize result interpretation among investigators.…”

Section: Discussionmentioning

confidence: 99%

Recovery from neutropenia can be predicted by the immature reticulocyte fraction several days before neutrophil recovery in autologous stem cell transplant recipients

Grazziutti

Lei

Miceli

et al. 2006

Bone Marrow Transplant

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The duration of neutropenia (absolute neutrophil count (ANC) p100/ll) identifies cancer patients at risk for infection. A test that precedes ANCX100/ll would be of clinical value. The immature reticulocyte fraction (IRF) reflects erythroid engraftment and hence a recovering marrow. We evaluated the IRF as predictor of marrow recovery among 90 myeloma patients undergoing their first and second (75 patients) melphalan-based autologous stem cell transplantation (Mel-ASCT). The time to IRF doubling (IRF-D) preceded ANCX100/ll in 99% of patients after the first Mel-ASCT by (mean7s.d.) 4.2371.96 days and in 97% of the patients after the second Mel-ASCT by 4.1171.95 days. We validated these findings in a group of 117 myeloma patients and 99 patients with various disorders undergoing ASCT with different conditioning regimens. We also compared the time to hypophosphatemia and to absolute monocyte countX100/ll to the time to ANCX100/ll. These markers were reached prior to this ANC end point in 55 and 25% of patients but were almost always preceded by IRF-D. We conclude that the IRF-D is a simple, inexpensive and widely available test that can predict marrow recovery several days before ANCX100/ll.

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Section: Discussionmentioning

confidence: 99%

Recovery from neutropenia can be predicted by the immature reticulocyte fraction several days before neutrophil recovery in autologous stem cell transplant recipients

Grazziutti

Lei

Miceli

et al. 2006

Bone Marrow Transplant

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“…The parameter has also been reported to distinguish iron deficiency anemia from anemia of chronic disease (34). A similar RMI parameter can be derived from the Sysmex R series' dedicated reticulocyte analyzers based on the fluorescence intensity of auramine 0 reticulocyte staining, which has also been reported to be an early predictor of bone marrow engraftment (3,9,19,22) and parallels the increase in circulating CD34+ cells following granulocyte colony-stim-0 1 9 9 5 Wiley-Liss, Inc.ulating factor (G-CSF) and granulocyte-macrophage colony-stimulating factor (GM-CSF) priming prior to peripheral stem cell harvesting (27,29). However, no information on the RMI and its relationship to standard hematologic red cell parameters in a large series of anemic patients has been reported.…”

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confidence: 99%

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confidence: 99%

Flow cytometric reticulocyte maturity index: A useful laboratory parameter of erythropoietic activity in anemia

1995

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Flow cytometric reticulocyte analysis is superior to manual reticulocyte counting with respect to precision and sensitivity. Furthermore, because the fluorescence intensity of reticulocytes is directly proportional to the erythrocyte RNA content, flow cytometric analysis using thiazole orange gives a quantitative reticulocyte maturity index (RMI). Previous studies have demonstrated that the RMI parameter is the earliest indicator of bone marrow engraftment following transplantation. In the present study, we analyzed the correlation of the RMI to standard red cell parameters, reticulocyte percentage, and absolute reticulocyte count in 41 3 anemic patients. The correlation of RMI to serum erythropoietin (Epo) and serum transferrin receptor (TfR) was analyzed in a subset of anemic blood samples. We found weak correlations between the RMI and hemoglobin (rZ = 0.0411, hematocrit (r2 = 0.0381, reticulocyte percentage (r2 = 0.0781, and absolute reticulocyte count (r2 = 0.087). Stronger correlations were observed between the RMI and Epo (r2 = 0.181) and the TfR (r2 = 0.191). The results indicate that the RMI represents a cost-effective measurement of erythropoietic activity and provides an additional parameter to classify anemic patients into categories of high and low erythropoietic activity, especially in hypoproductive anemias. o 1995 Wiley-Liss, Inc.Key terms: Erythropoiesis, erythrocyte, red cell, erythropoietin, transferrin receptor, thiazole orange It has recently been shown that flow cytometric reticulocyte analysis is more precise, more sensitive, and less costly than manual reticulocyte counting ( 5,6,8,10,15, 24,28). It is likely that this method will find widespread clinical use in the future for these reasons. In addition to accurate reticulocyte enumeration, because the measured fluorescence intensity is directly proportional to the amount of RNA in the immature erythrocytes, this method has the ability to quantitate reticulocyte maturity. Although reticulocyte maturation has been studied for over a century, only the flow cytometrically derived RMI appears to allow clinical utility (18). This quantitation of RNA in the reticulocytes using fluorescence intensity of thiazole orange-stained whole blood samples, termed the reticulocyte maturity index (RMI), has been shown to be an early predictor of bone marrow engraftment in transplant patients (2,1523). The parameter has also been reported to distinguish iron deficiency anemia from anemia of chronic disease (34). A similar RMI parameter can be derived from the Sysmex R series' dedicated reticulocyte analyzers based on the fluorescence intensity of auramine 0 reticulocyte staining, which has also been reported to be an early predictor of bone marrow engraftment (3,9,19,22) and parallels the increase in circulating CD34+ cells following granulocyte colony-stim-0 1 9 9 5 Wiley-Liss, Inc.ulating factor (G-CSF) and granulocyte-macrophage colony-stimulating factor (GM-CSF) priming prior to peripheral stem cell harvesting (27,29). However, no information on the ...

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“…Although reticulocyte counts performed by automated flow cytometric methods provide a good indicator of erythropoietic activity that may predict bone marrow regeneration, the duration, until increases in reticulocytes are seen, is usually later than or equal to that of neutrophils after transplantation. [4][5][6] Analysis of chimerism using fluorescence in situ hybridization (FISH) or polymerase chain reaction (PCR)-based methods can allow earlier demonstration of engraftment after transplantation, 7 but is costly and therefore unsuitable for routine monitoring.…”

Section: Introductionmentioning

confidence: 99%

Immature platelet fraction for prediction of platelet engraftment after allogeneic stem cell transplantation

Takami

Shibayama

Orito

et al. 2007

Bone Marrow Transplant

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Platelet regeneration represents an important and separate element in the engraftment process for allogeneic stem cell transplantation. Fully automated flow cytometry using blood cell counters now allows reliable quantification of reticulated platelets, expressed as the immature platelet fraction (IPF). We studied the kinetics of IPF in six patients grafted with allogeneic peripheral blood stem cell transplantation (PBSCT), 12 patients with bone marrow transplantation (BMT) and seven patients with cord blood transplantation (CBT). Preconditioning therapy caused an immediate and rapid fall in tri-lineage hematopoiesis. IPF rose transiently above 3% after a mean duration of 11 days post-PBSCT, 18 days post-BMT and 19 days post-CBT. This was 1, 4 and 13 days earlier than platelet engraftment, respectively. A linear correlation model showed a close association between the rise of IPF and tri-lineage engraftment after transplantation. IPF counting may thus provide an accessible measure of thrombopoietic activity, leading to early evaluation of marrow function and allowing monitoring of platelet regeneration.

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Evaluation of erythropoiesis after bone marrow transplantation: quantitative reticulocyte counting

Cited by 54 publications

References 6 publications

Recovery from neutropenia can be predicted by the immature reticulocyte fraction several days before neutrophil recovery in autologous stem cell transplant recipients

Recovery from neutropenia can be predicted by the immature reticulocyte fraction several days before neutrophil recovery in autologous stem cell transplant recipients

Flow cytometric reticulocyte maturity index: A useful laboratory parameter of erythropoietic activity in anemia

Immature platelet fraction for prediction of platelet engraftment after allogeneic stem cell transplantation

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