https://orcid.org/0000-0002-1957-3226
![A 57-year-old woman with no known medical history presented with fatigue and weakness. Her complete blood count showed white blood cell count, 413.6 × 109/L; hemoglobin level, 83 g/L; and platelet count, 244 × 109/L. A review of the peripheral blood smear showed 37% blasts with irregular nuclear contours, fine chromatin, and scant agranular cytoplasm. Other prominent findings included leukocytosis with left shift, mild basophilia, and eosinophilia (panels A-F; original magnification, ×1000). Flow cytometry of a peripheral blood specimen showed 34% blasts with the following immunophenotype: CD19+/CD10+/cytoCD22+/cytoCD79a+/TdT+/CD34partial+/CD20partial+/CD38(decreased+)/CD45 dim+/cytoCD3−/MPO−/κ−/λ− (panel G), diagnostic of B-cell acute lymphoblastic leukemia (B-ALL). Left-shifted myeloid maturation and eosinophilia were illustrated by flow cytometric immunophenotyping (panel G). Concurrent cytogenetics analysis showed an abnormal karyotype: 46,XX,t(9;22)(q34.1;q11.2)[17]/47,idem,+der(22)t(9;22)(q34.1;q11.2)[3]. Fluorescence in situ hybridization with a tricolor, dual-fusion BCR/ABL1 probe set revealed 77.5% cells with dual-fusion signals (1R1G2F2A) and 16.5% with an abnormal pattern (1G3F1A). Molecular testing by reverse transcription polymerase chain reaction showed a p210 BCR-ABL1 fusion transcript. Subsequent bone marrow biopsy showed 90% to 100% cellularity predominantly involved by B-ALL.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/139/2/10.1182_blood.2021013673/3/m_bloodbld2021013673f1.png?Expires=1763473830&Signature=tPZ~AK2gcwQcNhrr5TOJC--W4UJmQiVfO5NlwyOcQ-ykX91lu2CHfV-Mfk0Mwy8XBllkZQmLFjvKctcjLzUgFD372tRliM1B8Gvm~1wn25lRolELJPjt9J7nLgB1WpIbgbGcHG6~HNzHe7cArtz9O9X4vfWkoi6OwrEK-8TVYGKr9q~tETyM1RaDL~iWW8CsNFblT3LhaoeTASbylad16eXToik7CC3UiGtHjUY684A-qkS6S2FyEU2SIfa-CvSGUP2D8wJOW4B-TdASdKoIgaeH4DpVEruPxriumKerXcTZU22YydxpU~NIpAFMhUYqc6mH7dGFxOZ-nC0wHI2dJg__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
A 57-year-old woman with no known medical history presented with fatigue and weakness. Her complete blood count showed white blood cell count, 413.6 × 109/L; hemoglobin level, 83 g/L; and platelet count, 244 × 109/L. A review of the peripheral blood smear showed 37% blasts with irregular nuclear contours, fine chromatin, and scant agranular cytoplasm. Other prominent findings included leukocytosis with left shift, mild basophilia, and eosinophilia (panels A-F; original magnification, ×1000). Flow cytometry of a peripheral blood specimen showed 34% blasts with the following immunophenotype: CD19+/CD10+/cytoCD22+/cytoCD79a+/TdT+/CD34partial+/CD20partial+/CD38(decreased+)/CD45 dim+/cytoCD3−/MPO−/κ−/λ− (panel G), diagnostic of B-cell acute lymphoblastic leukemia (B-ALL). Left-shifted myeloid maturation and eosinophilia were illustrated by flow cytometric immunophenotyping (panel G). Concurrent cytogenetics analysis showed an abnormal karyotype: 46,XX,t(9;22)(q34.1;q11.2)[17]/47,idem,+der(22)t(9;22)(q34.1;q11.2)[3]. Fluorescence in situ hybridization with a tricolor, dual-fusion BCR/ABL1 probe set revealed 77.5% cells with dual-fusion signals (1R1G2F2A) and 16.5% with an abnormal pattern (1G3F1A). Molecular testing by reverse transcription polymerase chain reaction showed a p210 BCR-ABL1 fusion transcript. Subsequent bone marrow biopsy showed 90% to 100% cellularity predominantly involved by B-ALL.
The overall findings in this case were diagnostic of B-ALL. The clinical and laboratory features were highly suggestive of the B-lymphoid blast phase of chronic myeloid leukemia (CML). This case is an example of leukocytosis with myeloid left-shift maturation providing a clue for diagnosing the B-lymphoid blast phase in a patient with undiagnosed CML.
Figure edited by Amaris Shi, Clements High School, Sugar Land, TX.
A 57-year-old woman with no known medical history presented with fatigue and weakness. Her complete blood count showed white blood cell count, 413.6 × 109/L; hemoglobin level, 83 g/L; and platelet count, 244 × 109/L. A review of the peripheral blood smear showed 37% blasts with irregular nuclear contours, fine chromatin, and scant agranular cytoplasm. Other prominent findings included leukocytosis with left shift, mild basophilia, and eosinophilia (panels A-F; original magnification, ×1000). Flow cytometry of a peripheral blood specimen showed 34% blasts with the following immunophenotype: CD19+/CD10+/cytoCD22+/cytoCD79a+/TdT+/CD34partial+/CD20partial+/CD38(decreased+)/CD45 dim+/cytoCD3−/MPO−/κ−/λ− (panel G), diagnostic of B-cell acute lymphoblastic leukemia (B-ALL). Left-shifted myeloid maturation and eosinophilia were illustrated by flow cytometric immunophenotyping (panel G). Concurrent cytogenetics analysis showed an abnormal karyotype: 46,XX,t(9;22)(q34.1;q11.2)[17]/47,idem,+der(22)t(9;22)(q34.1;q11.2)[3]. Fluorescence in situ hybridization with a tricolor, dual-fusion BCR/ABL1 probe set revealed 77.5% cells with dual-fusion signals (1R1G2F2A) and 16.5% with an abnormal pattern (1G3F1A). Molecular testing by reverse transcription polymerase chain reaction showed a p210 BCR-ABL1 fusion transcript. Subsequent bone marrow biopsy showed 90% to 100% cellularity predominantly involved by B-ALL.
The overall findings in this case were diagnostic of B-ALL. The clinical and laboratory features were highly suggestive of the B-lymphoid blast phase of chronic myeloid leukemia (CML). This case is an example of leukocytosis with myeloid left-shift maturation providing a clue for diagnosing the B-lymphoid blast phase in a patient with undiagnosed CML.
Figure edited by Amaris Shi, Clements High School, Sugar Land, TX.
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![A 57-year-old woman with no known medical history presented with fatigue and weakness. Her complete blood count showed white blood cell count, 413.6 × 109/L; hemoglobin level, 83 g/L; and platelet count, 244 × 109/L. A review of the peripheral blood smear showed 37% blasts with irregular nuclear contours, fine chromatin, and scant agranular cytoplasm. Other prominent findings included leukocytosis with left shift, mild basophilia, and eosinophilia (panels A-F; original magnification, ×1000). Flow cytometry of a peripheral blood specimen showed 34% blasts with the following immunophenotype: CD19+/CD10+/cytoCD22+/cytoCD79a+/TdT+/CD34partial+/CD20partial+/CD38(decreased+)/CD45 dim+/cytoCD3−/MPO−/κ−/λ− (panel G), diagnostic of B-cell acute lymphoblastic leukemia (B-ALL). Left-shifted myeloid maturation and eosinophilia were illustrated by flow cytometric immunophenotyping (panel G). Concurrent cytogenetics analysis showed an abnormal karyotype: 46,XX,t(9;22)(q34.1;q11.2)[17]/47,idem,+der(22)t(9;22)(q34.1;q11.2)[3]. Fluorescence in situ hybridization with a tricolor, dual-fusion BCR/ABL1 probe set revealed 77.5% cells with dual-fusion signals (1R1G2F2A) and 16.5% with an abnormal pattern (1G3F1A). Molecular testing by reverse transcription polymerase chain reaction showed a p210 BCR-ABL1 fusion transcript. Subsequent bone marrow biopsy showed 90% to 100% cellularity predominantly involved by B-ALL.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/139/2/10.1182_blood.2021013673/3/m_bloodbld2021013673f1.png?Expires=1763473831&Signature=avict-oD6HosUoblIEj~M2uFOkGoit~oVIzfIGdLvQKVbPgvR7wEhIZw6u4aFvHVZ7eBTRM65EpD58OabM-tuxhFAD14RKYJ9QaauFObt6omnWzMj~h5RY2OVsFk1ObiABG~kJ3UZkjNUQKY9rVXVHANiHzYnxvvfmhrJg0suqDV3vPHVyHYH6DDcAQbhvrjfkGs-Im~pn8WHZDXWSvzVC-EgxSdThEGXYtWRku0QZXXZSOJHxgHoGBdylEhngU439iKjTwnog~AFEg8X0o3-qRMrIEo9dEn-o8P0KkI5HojmfAmRlVGacWRFW2t8EXqtf99o3pO2A0IPV24aheoCw__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
