Changes

24,927 bytes added , 13:04, 1 May 2024

no edit summary

Line 1: Line 1: −

~~Acute Myeloid Leukemia (AML) and Related Precursor Neoplasms~~

+

−

*[[~~Acute Myeloid Leukemia (AML) with Recurrent Genetic Abnormalities~~|~~AML with Recurrent Genetic Abnormalities]]~~

+

[[HAEM5:Table_of_Contents|Haematolymphoid Tumours (5th ed.)]]

−

**[[Acute Myeloid Leukemia (AML) with t(~~8;21)(q22;q22~~.1)~~; RUNX1-RUNX1T1|AML with t(8;21)(q22;q22.1); RUNX1-RUNX1T1~~]]

−

**[[Acute Myeloid Leukemia (AML) with inv(16)(p13.1q22) or t(16;16)(p13.1;q22); CBFB-MYH11|AML with with inv(16)(p13.1q22) or t(16;16)(p13.1;q22); CBFB-MYH11]]

−

*[[Acute Myeloid Leukemia (AML) with Myelodysplasia-Related Changes|AML with Myelodysplasia-Related Changes]]

−

**sub division

−

***sub-sub-sub division

+

−

== ~~Acute Myeloid Leukemia (AML) and Related Precursor Neoplasms ==~~

+

<blockquote class='blockedit'>{{Box-round|title=HAEM5 Conversion Notes|This page was converted to the new template on 2023-12-07. The original page can be found at [[HAEM4:Chronic Myeloid Leukemia (CML), BCR-ABL1 Positive]].

−

*[[~~Acute~~ Myeloid Leukemia (~~AML~~) ~~with Recurrent Genetic Abnormalities|AML with Recurrent Genetic Abnormalities~~]]

+

}}</blockquote>

−

~~- [[Acute Myeloid Leukemia~~ (~~AML) with t(8;21)(q22;q22~~.~~1); RUNX1-RUNX1T1|AML with t(8;21)(q22;q22.1); RUNX1-RUNX1T1]]~~

+

(General Instructions – The main focus of these pages is the clinically significant genetic alterations in each disease type. Use [https://www.genenames.org/ HUGO-approved gene names and symbols] (italicized when appropriate), [https://varnomen.hgvs.org/ HGVS-based nomenclature for variants], as well as generic names of drugs and testing platforms or assays if applicable. Please complete tables whenever possible and do not delete them (add N/A if not applicable in the table and delete the examples); to add (or move) a row or column to a table, click nearby within the table and select the > symbol that appears to be given options. Please do not delete or alter the section headings. The use of bullet points alongside short blocks of text rather than only large paragraphs is encouraged. Additional instructions below in italicized blue text should not be included in the final page content. Please also see [[Author_Instructions]] and [[Frequently Asked Questions (FAQs)|FAQs]] as well as contact your [[Leadership|Associate Editor]] or [mailto:CCGA@cancergenomics.org Technical Support])

−

~~- [~~[~~Acute Myeloid Leukemia (AML) with inv(16)(p13~~.~~1q22) or t(16;16)(p13~~.~~1;q22); CBFB~~-~~MYH11|AML with with inv(16)(p13.1q22) or t(16;16)(p13.1;q22); CBFB-MYH11~~]]

−

~~- [[Acute Promyelocytic Leukemia~~ (~~APL~~) ~~with PML-RARA]]~~

−

~~- [~~[~~Acute Myeloid Leukemia (AML) with t(9;11)(p21~~.~~3;q23~~.~~3); KMT2A-MLLT3|AML with t(9;11)(p21.3;q23.3); KMT2A~~-~~MLLT3~~]]

−

~~- [[Acute Myeloid Leukemia (AML) with t(6;9)(p23;q34~~.~~1); DEK-NUP214|AML with t~~(~~6;9)(p23;q34.1~~); ~~DEK-NUP214]]~~

−

~~- [[Acute Myeloid Leukemia~~ (~~AML) with inv(3)(q21.3q26.2~~) or ~~t(3;3)(q21.3;q26.2);GATA2~~, ~~MECOM|AML with inv(3)(q21~~.~~3q26~~.~~2) or t(3;3)(q21~~.~~3;q26~~.~~2);GATA2, MECOM]]~~

−

- [[~~Acute Myeloid Leukemia (AML) Megakaryoblastic with t(1;22)(p13.3;q13.1);RBM15-MKL1|AML Megakaryoblastic with t(1;22)(p13.3;q13.1);RBM15-MKL1~~]]

−

- [[~~Acute Myeloid Leukemia~~ (~~AML~~) ~~with BCR-ABL1~~|~~AML with BCR-ABL1~~]]

−

- [[~~Acute Myeloid Leukemia (AML) with Mutated NPM1~~|~~AML with Mutated NPM1~~]]

−

- [~~[Acute Myeloid Leukemia (AML) with Biallelic Mutations of CEBPA|AML with Biallelic Mutations of CEBPA~~]]

−

~~- [[Acute Myeloid Leukemia (AML~~) ~~with Mutated RUNX1|AML with Mutated RUNX1]]~~

−

*[[Acute Myeloid Leukemia (~~AML~~) ~~with Myelodysplasia-Related Changes|AML with Myelodysplasia-Related Changes]]~~

+

==Primary Author(s)*==

−

*[[Therapy-Related Myeloid Neoplasms]]

+

Jack Reid, MD (University of California, Irvine)

−

*[[Acute Myeloid Leukemia (~~AML~~)~~, Not Otherwise Specified|AML, Not Otherwise Specified]]~~

+

Mark Evans, MD (University of California, Irvine)

−

- ~~[[Acute Myeloid Leukemia~~ (~~AML~~) ~~with Minimal Differentiation|AML with Minimal Differentiation]]~~

+

Fabiola Quintero-Rivera, MD (University of California, Irvine)

−

~~- [[Acute Myeloid Leukemia (AML) without Maturation|AML without Maturation]]~~

−

~~- [[Acute Myeloid Leukemia (AML) with Maturation|AML with Maturation]]~~

−

~~- [[Acute Myelomonocytic Leukemia]]~~

−

~~- [[Acute Monoblastic and Monocytic Leukemia]]~~

−

~~- [[Pure Erythroid Leukemia]]~~

−

~~- [[Acute Megakaryoblastic Leukemia (AMKL)]]~~

−

~~- [[Acute Basophilic Leukemia]]~~

−

~~- [[Acute Panmyelosis with Myelofibrosis]]~~

−

*[[Myeloid Sarcoma]]

+

__TOC__

−

*[[Myeloid Proliferations Associated with Down Syndrome]]

+

==Cancer Category / Type==

−

~~- [[Transient Abnormal Myelopoiesis (TAM) Associated with Down Syndrome]]~~

+

Myeloproliferative neoplasm

−

~~- [[Myeloid Leukemia Associated with Down Syndrome]]~~

−

*[[Blastic Plasmacytoid Dendritic Cell Neoplasm]]

+

==Cancer Sub-Classification / Subtype==

−

*[[Acute Leukemias of Ambiguous Lineage]]

+

Not applicable.

−

~~- [[Acute Undifferentiated Leukemia]]~~

+

==Definition / Description of Disease==

−

~~- [[Mixed Phenotype Acute Leukemia (MPAL) with t(9;22)(q34.1;q11.2); BCR-ABL1]]~~

−

~~- [[Mixed Phenotype Acute Leukemia (MPAL) with t(v;11q23.3); KMT2A Rearranged]]~~

−

~~- [[Mixed Phenotype Acute Leukemia (MPAL), B~~/~~Myeloid, Not Otherwise Specified]]~~

−

~~- [[Mixed Phenotype Acute Leukemia (MPAL), T/Myeloid, Not Otherwise Specified]]~~

−

~~- [[Mixed-Phenotype Acute Leukemia, Not Otherwise Specified (NOS), Rare Types]]~~

−

~~- [[Acute Leukemias~~ of ~~Ambiguous Lineage, Not Otherwise Specified (NOS)]]~~

−

*[[Myeloid ~~Neoplasms with Germline Predisposition]]~~

+

Chronic myeloid leukemia (CML) is a myeloproliferative neoplasm that is characterized by clonal expansion of predominantly granulocytic proliferation (neutrophils, eosinophils and basophils). The majority of the patients with CML are known to have a gene rearrangement called the Philadelphia Chromosome, which is a balanced genetic translocation t(9;22)(q34.1;q11.2) involving a fusion of the Abelson gene (ABL1) from chromosome 9q34 with the breakpoint cluster region (BCR) gene on chromosome 22q11.2. Althought 80% of the clonal evolution in CML cases can be attributed to classic Ph chromosome, secondary cytogenetic aberrations can be seen such as isochromosome 17q, gain of chromosome 8 or 19. ML was first recognized in 1845<ref>{{Cite journal|last=Jm|first=Goldman|last2=Jv|first2=Melo|date=2003|title=Chronic Myeloid Leukemia--Advances in Biology and New Approaches to Treatment|url=https://pubmed.ncbi.nlm.nih.gov/14534339/|language=en|pmid=14534339}}</ref>. Nowell and Hungerford in 1960, who coined the term Philadelphia Chromosome after realizing consistent chromosomal abnormality in leukemic cells.<ref>{{Cite journal|last=Nowell|first=Peter C.|date=2007|title=Discovery of the Philadelphia chromosome: a personal perspective|url=https://www.ncbi.nlm.nih.gov/pmc/articles/PMC1934591/|journal=Journal of Clinical Investigation|volume=117|issue=8|pages=2033–2035|doi=10.1172/JCI31771|issn=0021-9738|pmc=1934591|pmid=17671636}}</ref> Later in 1973, the characteristic cytogenetic feature of CML was identified: reciprocal translocation of t(9;22)(q34.1;q11.2).<ref>{{Cite journal|last=Jd|first=Rowley|date=1973|title=Letter: A New Consistent Chromosomal Abnormality in Chronic Myelogenous Leukaemia Identified by Quinacrine Fluorescence and Giemsa Staining|url=https://pubmed.ncbi.nlm.nih.gov/4126434/|language=en|pmid=4126434}}</ref> CML has the capacity to expand in both myeloid and lymphoid lineages. However, expansion is predominantly in the granulocyte compartment of the myeloid lineages in the bone marrow.<ref>{{Cite journal|last=S|first=Faderl|last2=M|first2=Talpaz|last3=Z|first3=Estrov|last4=S|first4=O'Brien|last5=R|first5=Kurzrock|last6=Hm|first6=Kantarjian|date=1999|title=The Biology of Chronic Myeloid Leukemia|url=https://pubmed.ncbi.nlm.nih.gov/10403855/|language=en|pmid=10403855}}</ref> In the previous WHO 4th edition, CML was be divided into 3 phases of disease: chronic phase, accelerated phase and blastic phase. Currently, in the revised classification of CML, AP at diagnosis or during treatment has been omitted and replaced by recognising only the chronic and blast phases

−

~~- [[Acute Myeloid Leukaemia with Germline CEBPA Mutation]]~~

+

==Synonyms / Terminology==

−

~~- [[Myeloid Neoplasms with Germline DDX41 Mutation]]~~

−

~~- [[Myeloid Neoplasms with Germline RUNX1 Mutation]]~~

−

~~- [[Myeloid Neoplasms with Germline ANKRD26 Mutation]]~~

−

~~- [[Myeloid Neoplasms with Germline ETV6 Mutation]]~~

−

~~- [[Myeloid Neoplasms with Germline GATA2 Mutation]]~~

−

~~== Myelodysplastic Syndromes (MDS) ==~~

+

Formerly chronic myelogenous leukemia or chronic granulocytic leukemia

−

*[[Myelodysplastic Syndrome (MDS) with Single Lineage Dysplasia|MDS with Single Lineage Dysplasia]]

−

*[[Myelodysplastic Syndrome with Ring Sideroblasts (MDS-RS)|MDS with Ring Sideroblasts (MDS-RS)]]

−

*[[Myelodysplastic Syndrome with Ring Sideroblasts and Multilineage Dysplasia|MDS with Ring Sideroblasts and Multilineage Dysplasia]]

−

*[[Myelodysplastic Syndrome (MDS) with Multilineage Dysplasia|MDS with Multilineage Dysplasia]]

−

*[[Myelodysplastic Syndrome (MDS) with Excess Blasts|MDS with Excess Blasts]]

−

*[[Myelodysplastic Syndrome (MDS) with Isolated del(5q)|MSD with Isolated del(5q)]]

−

*[[Myelodysplastic Syndrome (MDS), Unclassifiable|MDS, Unclassifiable]]

−

*[[Refractory Cytopenia of Childhood]]

−

== ~~Myeloproliferative Neoplasms (MPN)~~ ==

+

==Epidemiology / Prevalence==

−

*[[Chronic Myeloid Leukemia (CML), BCR-ABL1 Positive]]

−

*[[Chronic Neutrophilic Leukemia (CNL)]]

−

*[[Polycythemia Vera (PV)]]

−

*[[Primary Myelofibrosis (PMF)]]

−

*[[Essential Thrombocythemia (ET)]]

−

*[[Chronic Eosinophilic Leukemia, Not Otherwise Specified]]

−

*[[Myeloproliferative Neoplasm (MPN), Unclassifiable]]

−

== ~~Myelodysplastic~~/~~Myeloproliferative Neoplasms (MDS~~/~~MPN)~~ ==

+

Global annual incidence of CML is 1-2 cases per 100,000 population. CML has male predominance with male to female ratio of 1.4:1. The prevalence of CML is increasing due to successful Tyrosine kinase inhibitor (TKI) therapy. Predilection of CML among certain ethnic groups has not been reported.<ref>{{Cite journal|last=Jv|first=Melo|last2=De|first2=Gordon|last3=Nc|first3=Cross|last4=Jm|first4=Goldman|date=1993|title=The ABL-BCR Fusion Gene Is Expressed in Chronic Myeloid Leukemia|url=https://pubmed.ncbi.nlm.nih.gov/8417787/|language=en|pmid=8417787}}</ref> Regional variations in age at diagnosis and overall survival among patients with chronic myeloid leukemia from low and middle income countries.<ref>{{Cite journal|last=Am|first=Mendizabal|last2=P|first2=Garcia-Gonzalez|last3=Ph|first3=Levine|date=2013|title=Regional Variations in Age at Diagnosis and Overall Survival Among Patients With Chronic Myeloid Leukemia From Low and Middle Income Countries|url=https://pubmed.ncbi.nlm.nih.gov/23411044/|language=en|pmid=23411044}}</ref> The median age of patients diagnosed with CML is 66 years according to Surveillance, Epidemiology, and End Results (SEER) program and Medical Research Council (MRC) data. Although the etiology of CML is largely unknown, cases of CML have been reported in association with radiation exposure. No studies have shown any genetic inheritance of CML.

−

*[[Chronic Myelomonocytic Leukemia (CMML)]]

−

*[[Atypical Chronic Myeloid Leukemia ~~(aCML), BCR-ABL1 Negative]]~~

−

*[[Juvenile Myelomonocytic Leukemia (JMML)]]

−

*[[Myelodysplastic/~~Myeloproliferative Neoplasms with Ring Sideroblasts and Thrombocytosis (MDS~~/~~MPN-RS-T)~~|~~MDS~~/~~MPN~~ with ~~Ring Sideroblasts~~ and ~~Thrombocytosis~~ (~~MDS/MPN-RS-T~~)]]

−

*[[Myelodysplastic/Myeloproliferative Neoplasms (~~MDS/MPN~~), ~~Unclassifiable|MDS/MPN, Unclassifiable]]~~

+

==Clinical Features==

+

Put your text here and fill in the table (''Instruction: Can include references in the table. Do not delete table.'')

+

{| class="wikitable"

+

|'''Signs and Symptoms'''

+

|EXAMPLE: Asymptomatic (incidental finding on complete blood counts)

+

EXAMPLE: B-symptoms (weight loss, fever, night sweats)

+

EXAMPLE: Lymphadenopathy (uncommon)

+

|-

+

|'''Laboratory Findings'''

+

|EXAMPLE: Cytopenias

+

EXAMPLE:

+

{| class="wikitable"

+

|'''Signs and Symptoms'''

+

|EXAMPLE: Asymptomatic (incidental finding on complete blood counts)

+

EXAMPLE: B-symptoms (weight loss, fever, night sweats)

−

=~~= Mature B~~-~~Cell Neoplasms ==~~

+

EXAMPLE: Fatigue

−

*[[Chronic Lymphocytic Leukemia/~~Small Lymphocytic Lymphoma]]~~

−

~~- [[Monoclonal B-cell Lymphocytosis]]~~

−

*[[B-~~cell Prolymphocytic Leukemia]]~~

+

EXAMPLE: Lymphadenopathy (uncommon)

+

|-

+

|'''Laboratory Findings'''

+

|EXAMPLE: Cytopenias

−

*[[Splenic Marginal Zone Lymphoma]]

+

EXAMPLE: Lymphocytosis (low level)

+

|}

−

*[[Hairy Cell Leukemia]]

−

*[[Splenic B-~~cell Lymphoma~~/Leukemia, ~~Unclassifiable]]~~

+

<blockquote class='blockedit'>{{Box-round|title=v4:Clinical Features|The content below was from the old template. Please incorporate above.}}

−

- ~~[[Splenic Diffuse Red Pulp Small B-cell Lymphoma]]~~

+

Approximately 50% of the patients who are diagnosed with CML are asymptomatic and diagnosed during the routine blood tests.<ref name=":0">Silver RT. Molecular Biology of CML. In: Kufe DW, Pollock RE, Weichselbaum RR, et al., editors. Holland-Frei Cancer Medicine. 6th edition. Hamilton (ON): BC Decker; 2003. Available from: <nowiki>https://www.ncbi.nlm.nih.gov/books/NBK13554/</nowiki></ref> CML is a hematological disease that occurs predominantly in adults but in rare cases, it can occur in the pediatric population.<ref>{{Cite journal|last=Am|first=Mendizabal|last2=P|first2=Garcia-Gonzalez|last3=Ph|first3=Levine|date=2013|title=Regional Variations in Age at Diagnosis and Overall Survival Among Patients With Chronic Myeloid Leukemia From Low and Middle Income Countries|url=https://pubmed.ncbi.nlm.nih.gov/23411044/|language=en|pmid=23411044}}</ref> The onset of CML is insidious. Patients with CML usually experience dragging sensation of the abdomen due to splenomegaly. The clinical hallmark of CML is the uncontrolled proliferation of mature and maturing granulocytes at all stages of maturation: metamyelocytes, myelocytes, promyelocytes, and myeloblasts. Patients with CML usually begin with the initial chronic phase before entering the terminal blastic phase and 60-80% of the patients go through accelerated phase before reaching the terminal blastic phase. In chronic phase, CML patients show abnormal routine blood tests with clinical symptoms such as unintentional weight loss, loss of appetite, satiety, fatigue, insomnia and palpable splenomegaly. In rare cases, hyperviscosity syndrome can be a manifestation with a wide spectrum of features such as priapism, tinnitus, hearing loss, cerebral accidents and blindness. In the blastic phase, CML leukemic cells resemble acute leukemic cells morphologically. CNS and lymph node involvement are notable in the blastic phase of CML. If untreated, CML patients will progress to the terminal blastic phase in 3 to 5 years.

−

~~- [[Hairy Cell Leukemia Variant]]~~

−

*[[Lymphoplasmacytic Lymphoma]]

+

</blockquote>

−

~~- [[Waldenstrom Macroglobulinemia]]~~

+

==Sites of Involvement==

−

*[[IgM Monoclonal Gammopathy of ~~Undetermined Significance]]~~

+

Spleen is known to be the most common site of involvement as patients with CML usually present with splenomegaly. Literature has shown that bone marrow is always involved in patients with CML.

−

*[[~~Heavy Chain Diseases~~]]

+

==Morphologic Features==

−

- ~~[[Mu Heavy Chain Disease]]~~

+

[[File:CML 1.jpg|thumb|Chronic Myeloid Leukemia. Image courtesy of Jack Reid, MD]]

−

- ~~[[Gamma Heavy Chain Disease]]~~

+

Morphologically, peripheral blood smear shows the classic features of chronic-phase CML: granulocytic leukocytosis with left shift, neutrophilia, no increase in blasts, myelocyte “bulge” and basophilia.<ref>Vardiman JW, et al., (2016). Chronic myeloid leukaemia, BCR-ABL1-positive, in World Health Organization Classification of Tumours of Haematopoietic and Lymphoid Tissues, Revised 4th edition. Swerdlow SH, Campo E, Harris NL, et al., Editors. IARC Press: Lyon, France, p30-36.</ref> Granulocytes seen in CML patients usually lack dysplastic features. In bone marrow, the aspirate smear shows classic features of CML: marked increase in neutrophils and precursors with a myeloid: erythroid ratio of > 10:1 and small hypolobated megakaryocytes. CML can sometimes present with thrombocytosis in peripheral blood smear, mimicking essential thrombocythemia (ET). Most of the time, primary myelofibrosis (PMF) share overlapping morphological features with CML in the peripheral blood; one distinguishing feature is that the megakaryocyte morphology in PMF is large, bizarre, and hyperchromatic, which is the feature not seen in the CML.

−

- ~~[[Alpha Heavy Chain Disease]]~~

−

*[[Plasma Cell Neoplasms]]

+

==Immunophenotype==

−

~~- [[Non-IgM Monoclonal Gammopathy of Undetermined Signiﬁcance]]~~

−

~~- [[Plasma Cell Myeloma]]~~

−

~~- [[Plasma Cell Myeloma Variants]]~~

−

~~- [[Plasmacytoma]]~~

−

~~- [[Monoclonal Immunoglobulin Deposition Diseases]]~~

−

~~- [[Primary Amyloidosis]]~~

−

~~- [[Light Chain and Heavy Chain Deposition Disease]]~~

−

~~- [[Plasma Cell Neoplasms with Associated Paraneoplastic Syndrome]]~~

−

~~- [[POEMS Syndrome]]~~

−

~~- [[TEMPI Syndrome]]~~

−

*[[Extranodal Marginal Zone Lymphoma of ~~Mucosa~~-~~Associated Lymphoid Tissue~~ (~~MALT Lymphoma~~)]]

+

The role of immunohistochemistry is minimal in diagnosing CML. CML usually shows blastic markers (CD 34, CD 117, TdT), which can be useful to confirm extramedullary (splenic involvement with blastic transformation). Lineage-specific markers (MPO, lysosome, CD42b, CD79a, PAX5, CD3) are helpful in distinguishing among myeloid, lymphoid or megakaryocytic transformation.

−

*[[Nodal Marginal Zone Lymphoma]]

+

{| class="wikitable sortable"

−

- ~~[[Paediatric Nodal Marginal Zone Lymphoma]]~~

+

|-

+

!Finding!!Marker

+

|-

+

|Positive||CD34

+

|-

+

|Positive||CD117

+

|-

+

|

+

Positive

+

|Tdt

+

|}

−

*[[Follicular Lymphoma]]

+

==Chromosomal Rearrangements (Gene Fusions)==

−

~~- [[Testicular Follicular Lymphoma]]~~

−

~~- [[In Situ Follicular Neoplasia]]~~

−

~~- [[Duodenal-Type Follicular Lymphoma]]~~

−

*[[Paediatric-Type Follicular Lymphoma]]

+

Put your text here and fill in the table

−

*[[Large B-~~cell Lymphoma with IRF4~~ Rearrangement]]

+

{| class="wikitable sortable"

+

|-

+

!Chromosomal Rearrangement!!Genes in Fusion (5’ or 3’ Segments)!!Pathogenic Derivative!!Prevalence

+

!Diagnostic Significance (Yes, No or Unknown)

+

!Prognostic Significance (Yes, No or Unknown)

+

!Therapeutic Significance (Yes, No or Unknown)

+

!Notes

+

|-

+

|EXAMPLE: t(9;22)(q34;q11.2)||EXAMPLE: 3'ABL1 / 5'BCR||EXAMPLE: der(22)||EXAMPLE: 20% (COSMIC)

+

EXAMPLE: 30% (add reference)

+

|Yes

+

|No

+

|Yes

+

|EXAMPLE:

−

*[[Primary Cutaneous Follicle Centre Lymphoma]]

+

The t(9;22) is diagnostic of CML in the appropriate morphology and clinical context (add reference). This fusion is responsive to targeted therapy such as Imatinib (Gleevec) (add reference).

+

|}

+

−

*[[Mantle Cell Lymphoma]]

+

<blockquote class='blockedit'>{{Box-round|title=v4:Chromosomal Rearrangements (Gene Fusions)|The content below was from the old template. Please incorporate above.}}

−

- ~~[[Leukemic Non-Nodal Mantle Cell Lymphoma]]~~

−

~~- [[In Situ Mantle Cell Neoplasia]]~~

−

*[[Diffuse Large B-cell ~~Lymphoma, Not Otherwise Specified]]~~

+

CML is the first cancer that is known to be linked to a specific genetic abnormality, namely the balanced chromosomal translocation known as Philadelphia Chromosome. A focal gene area of BCR (Breakpoint Cluster Region) from chromosome 22 is fused with another gene ABL (Tyrosine protein kinase ABL) that is located on chromosome 9. The chimeric oncogene BCR-ABL is the central to the pathology of CML because ABL carries a domain that is capable of phosphorylating tyrosine residues, activating a cascade of proteins that control the cell cycle. It was reported that 90% - 95% of the CML in chronic phase shows characteristic t(9;22)(q34;q11.2) reciprocal translocation that results in the Ph chromosome. This balanced translocation leads to the formation of the ''BCR/ABL'' fusion gene on chromosome 22 and a reciprocal ''ABL/BCR'' fusion gene on chromosome 9. Studies has shown that the latter gene ''ABL/BCR'' fusion gene does not seem to have any crucial role in CML and no ABL/BCR protein has been found.

−

*[[T-~~cell~~/~~Histiocyte-Rich Large B-cell Lymphoma]]~~

+

{| class="wikitable sortable"

+

|-

+

!Chromosomal Rearrangement!!Genes in Fusion (5’ or 3’ Segments)!!Prevalence

+

|-

+

|t(9;22)(q34.1;q11.2)||3'ABL1 / 5'BCR||More than 90%

+

|}

+

</blockquote>

−

*[[Primary Diffuse Large B-cell Lymphoma of the CNS]]

−

*[[Primary Cutaneous Diffuse Large B-~~cell Lymphoma~~, ~~Leg Type]]~~

+

<blockquote class='blockedit'>{{Box-round|title=v4:Clinical Significance (Diagnosis, Prognosis and Therapeutic Implications).|Please incorporate this section into the relevant tables found in:

+

* Chromosomal Rearrangements (Gene Fusions)

+

* Individual Region Genomic Gain/Loss/LOH

+

* Characteristic Chromosomal Patterns

+

* Gene Mutations (SNV/INDEL)}}

−

*[[EBV-Positive Diffuse Large B-cell Lymphoma, Not Otherwise Specified (NOS)]]

+

'''Diagnosis:'''

−

*[[EBV-~~Positive Mucocutaneous Ulcer]]~~

+

Currently four FDA approved tyrosine kinase inhibitors (TKIs) - imatinib, nilotinib, dasatinib and bosutinib - are the first line of treatment for patients with newly diagnosed CML in chronic phase (CML-CP).<ref>{{Cite journal|last=Ja|first=Kennedy|last2=G|first2=Hobbs|date=2018|title=Tyrosine Kinase Inhibitors in the Treatment of Chronic-Phase CML: Strategies for Frontline Decision-making|url=https://pubmed.ncbi.nlm.nih.gov/29687320/|language=en|doi=10.1007/s11899-018-0449-7|pmc=PMC6023770|pmid=29687320}}</ref> For many years, inhibitors of the specific BCR-ABL1 tyrosine kinase are considered to be the most effective targeted therapy. A subset of CML patients can demonstrate resistance to TKI therapy through mutations in ABL1 and other mechanisms. The culprit of the resistance to TKI therapy can be attributed to so-called leukemic stem cells (LSCs), pluripotent BCR-ABL1+ progenitors that are largely quiescent.<ref>{{Cite journal|last=S|first=Tabarestani|last2=A|first2=Movafagh|date=2016|title=New Developments in Chronic Myeloid Leukemia: Implications for Therapy|url=https://pubmed.ncbi.nlm.nih.gov/27366312/|language=en|doi=10.17795/ijcp-3961|pmc=PMC4922205|pmid=27366312}}</ref> Therefore, understanding of signaling pathways related to survival of LSCs may be helpful.

−

*[[Diffuse Large B-~~cell Lymphoma Associated~~ with ~~Chronic Inflammation]]~~

+

'''Prognosis''': Acquired resistance to imatinib therapy , mostly with mutation in BCR-ABL kinase domain, is known to be associated with poor prognosis.<ref>{{Cite journal|last=S|first=Branford|last2=Z|first2=Rudzki|last3=S|first3=Walsh|last4=I|first4=Parkinson|last5=A|first5=Grigg|last6=J|first6=Szer|last7=K|first7=Taylor|last8=R|first8=Herrmann|last9=Jf|first9=Seymour|date=2003|title=Detection of BCR-ABL Mutations in Patients With CML Treated With Imatinib Is Virtually Always Accompanied by Clinical Resistance, and Mutations in the ATP Phosphate-Binding Loop (P-loop) Are Associated With a Poor Prognosis|url=https://pubmed.ncbi.nlm.nih.gov/12623848/|language=en|pmid=12623848}}</ref> Five prognostic factors were shown to be associated with major cytogenetic response: the absence of blasts in peripheral blood, a hemoglobin level of more than 12 g per deciliter, the presence of less than 5 percent blasts in marrow, a time from diagnosis of CML to start of treatment of less than one year, and a history of cytogenetic relapse during interferon therapy.<ref>{{Cite journal|last=H|first=Kantarjian|last2=C|first2=Sawyers|last3=A|first3=Hochhaus|last4=F|first4=Guilhot|last5=C|first5=Schiffer|last6=C|first6=Gambacorti-Passerini|last7=D|first7=Niederwieser|last8=D|first8=Resta|last9=R|first9=Capdeville|date=2002|title=Hematologic and Cytogenetic Responses to Imatinib Mesylate in Chronic Myelogenous Leukemia|url=https://pubmed.ncbi.nlm.nih.gov/11870241/|language=en|pmid=11870241}}</ref>

−

- ~~[[Fibrin~~-Associated ~~Diffuse Large B~~-~~cell Lymphoma]]~~

−

*[[Lymphomatoid Granulomatosis]]

+

'''Therapeutic implication''': Studies have shown that median survival

−

*[[Primary Mediastinal (~~Thymic~~) ~~Large B~~-~~cell Lymphoma]]~~

+

Complete cytogenetic response is defined as 0% of Philadelphia-chromosome (Ph)-positive cells in metaphase in bone marrow.<ref>{{Cite journal|last=J|first=Cortes|last2=A|first2=Quintás-Cardama|last3=Hm|first3=Kantarjian|date=2011|title=Monitoring Molecular Response in Chronic Myeloid Leukemia|url=https://pubmed.ncbi.nlm.nih.gov/20960522/|language=en|doi=10.1002/cncr.25527|pmc=PMC4969001|pmid=20960522}}</ref>

−

*[[Intravascular Large B-cell Lymphoma]]

+

</blockquote>

+

==Individual Region Genomic Gain / Loss / LOH==

−

*[[~~ALK~~-~~Positive Large B~~-~~cell Lymphoma]~~]

+

Put your text here and fill in the table (''Instructions: Includes aberrations not involving gene fusions. Can include references in the table. Can refer to CGC workgroup tables as linked on the homepage if applicable. Do not delete table.'')

+

{| class="wikitable sortable"

+

|-

+

!Chr #!!Gain / Loss / Amp / LOH!!Minimal Region Genomic Coordinates [Genome Build]!!Minimal Region Cytoband

+

!Diagnostic Significance (Yes, No or Unknown)

+

!Prognostic Significance (Yes, No or Unknown)

+

!Therapeutic Significance (Yes, No or Unknown)

+

!Notes

+

|-

+

|EXAMPLE:

+

7

+

|EXAMPLE: Loss

+

|EXAMPLE:

+

chr7:1-159,335,973 [hg38]

+

|EXAMPLE:

+

chr7

+

|EXAMPLE: Yes

+

|EXAMPLE: Yes

+

|EXAMPLE: No

+

|EXAMPLE:

+

Presence of monosomy 7 (or 7q deletion) is sufficient for a diagnosis of AML with MDS-related changes when there is ≥20% blasts and no prior therapy (add reference). Monosomy 7/7q deletion is associated with a poor prognosis in AML (add reference).

+

|-

+

|EXAMPLE:

+

8

+

|EXAMPLE: Gain

+

|EXAMPLE:

+

chr8:1-145,138,636 [hg38]

+

|EXAMPLE:

+

chr8

+

|EXAMPLE: No

+

|EXAMPLE: No

+

|EXAMPLE: No

+

|EXAMPLE:

−

*[~~[Plasmablastic Lymphoma]~~]

+

{| class="wikitable sortable"

+

|-

+

!Chr #!!Gain / Loss / Amp / LOH!!Minimal Region Genomic Coordinates [Genome Build]!!Minimal Region Cytoband

+

!Diagnostic Significance (Yes, No or Unknown)

+

!Prognostic Significance (Yes, No or Unknown)

+

!Therapeutic Significance (Yes, No or Unknown)

+

!Notes

+

|-

+

|EXAMPLE:

−

*[[Primary Effusion Lymphoma]]

+

7

+

|EXAMPLE: Loss

+

|EXAMPLE:

−

*[[HHV8-~~Associated Lymphoproliferative Disorders]]~~

+

chr7:1- 159,335,973 [hg38]

−

~~- [[Multicentric Castleman Disease]]~~

+

|EXAMPLE:

−

~~- [~~[~~HHV8-Positive Diffuse Large B-cell Lymphoma, Not Otherwise Specified (NOS)]~~]

−

~~- [[HHV8~~-~~Positive Germinotropic Lymphoproliferative Disorder]]~~

−

*[[Burkitt Lymphoma]]

+

chr7

+

|Yes

+

|Yes

+

|No

+

|EXAMPLE:

−

*[[Burkitt-~~Like Lymphoma~~ with ~~11q Aberration]]~~

+

Presence of monosomy 7 (or 7q deletion) is sufficient for a diagnosis of AML with MDS-related changes when there is ≥20% blasts and no prior therapy (add reference). Monosomy 7/7q deletion is associated with a poor prognosis in AML (add reference).

+

|-

+

|EXAMPLE:

−

*[[High-Grade B-cell Lymphoma]]

+

8

−

~~- [[High~~-~~Grade B-cell Lymphoma with MYC and BCL2 and~~/~~or BCL6 Rearrangements]]~~

+

|EXAMPLE: Gain

−

- ~~[[High-Grade B-cell Lymphoma, Not Otherwise Specified (NOS)]]~~

+

|EXAMPLE:

−

*[[B-~~cell Lymphoma~~, ~~Unclassifiable~~, ~~with Features Intermediate Between Diffuse Large B~~-~~cell Lymphoma and Classic Hodgkin Lymphoma]]~~

+

chr8:1-145,138,636 [hg38]

+

|EXAMPLE:

−

=~~= Mature T- and NK-cell Neoplasms ==~~

+

chr8

−

*[[T-~~cell Prolymphocytic Leukemia]]~~

+

|No

+

|No

+

|No

+

|EXAMPLE:

−

*[[T-cell Large Granular Lymphocytic Leukemia]]

+

Common recurrent secondary finding for t(8;21) (add reference).

+

|}

−

*[[Chronic Lymphoproliferative Disorder of NK Cells]]

+

<blockquote class='blockedit'>{{Box-round|title=v4:Genomic Gain/Loss/LOH|The content below was from the old template. Please incorporate above.}}

−

*[[Aggressive NK-cell Leukemia]]

+

Not Applicable.

+

</blockquote>

+

==Characteristic Chromosomal Patterns==

−

*[[EBV-Positive T-cell and NK-~~cell Lymphoproliferative Diseases~~ of ~~Childhood]]~~

+

Put your text here (''EXAMPLE PATTERNS: hyperdiploid; gain of odd number chromosomes including typically chromosome 1, 3, 5, 7, 11, and 17; co-deletion of 1p and 19q; complex karyotypes without characteristic genetic findings; chromothripsis. Do not delete table.'')

−

- ~~[[Systemic EBV~~-~~Positive T~~-~~cell Lymphoma of Childhood]]~~

+

{| class="wikitable sortable"

−

- ~~[[Chronic Active EBV Infection~~ of T- and NK-~~cell Type, Systemic Form]]~~

+

|-

−

- ~~[[Hydroa Vacciniforme~~-~~Like Lymphoproliferative Disorder]]~~

+

!Chromosomal Pattern

−

- ~~[[Severe Mosquito Bite Allergy]]~~

+

!Diagnostic Significance (Yes, No or Unknown)

+

!Prognostic Significance (Yes, No or Unknown)

+

!Therapeutic Significance (Yes, No or Unknown)

+

!Notes

+

|-

+

|EXAMPLE:

+

Co-deletion of 1p and 18q

+

|EXAMPLE: Yes

+

|EXAMPLE: No

+

|EXAMPLE: No

+

|EXAMPLE:

−

*[[Adult T-~~cell Leukemia~~/~~Lymphoma]]~~

+

{| class="wikitable sortable"

+

|-

+

!Chromosomal Pattern

+

!Diagnostic Significance (Yes, No or Unknown)

+

!Prognostic Significance (Yes, No or Unknown)

+

!Therapeutic Significance (Yes, No or Unknown)

+

!Notes

+

|-

+

|EXAMPLE:

−

*[[Extranodal NK/~~T-cell Lymphoma, Nasal Type]]~~

+

Co-deletion of 1p and 18q

+

|Yes

+

|No

+

|No

+

|EXAMPLE:

−

*[[Intestinal T-cell Lymphoma]]

+

See chromosomal rearrangements table as this pattern is due to an unbalanced derivative translocation associated with oligodendroglioma (add reference).

−

~~- [[Enteropathy-Associated T-cell Lymphoma]]~~

+

|}

−

~~- [[Monomorphic Epitheliotropic Intestinal T-cell Lymphoma]]~~

−

~~- [[Intestinal T-cell Lymphoma, Not Otherwise Specified~~ (~~NOS~~)]]

−

~~- [[Indolent T-cell Lymphoproliferative Disorder of the Gastrointestinal Tract]]~~

−

*[[Hepatosplenic T-~~cell Lymphoma]]~~

+

<blockquote class='blockedit'>{{Box-round|title=v4:Characteristic Chromosomal Aberrations / Patterns|The content below was from the old template. Please incorporate above.}}

−

*[[Subcutaneous Panniculitis-Like T-cell Lymphoma]]

+

Atypical chronic myeloid leukemia (aCML) is a subtype of myelodysplastic/myeloproliferative neoplasm that lacks Philadelphia chromosome or rearrangements of PDGFRA, PDGFRB, or FGFR1. This hematological disorder has a considerable overlapping clinicopathological features with CML and CMML. It differs from CML by older median age, lower level of granulocytosis, multilineage dysplasia and lack of basophilia. Up until now, no cytogenetic changes have been associated with aCML. In peripheral blood smear, aCML typically shows granulocytic leukocytosis with striking neutrophil dysplasia (nuclear hyposegmentation and hypogranularity).

−

*[[Mycosis Fungoides]]

+

</blockquote>

+

==Gene Mutations (SNV / INDEL)==

−

*[~~[Sézary Syndrome]~~]

+

Put your text here and fill in the table (''Instructions: This table is not meant to be an exhaustive list; please include only genes/alterations that are recurrent and common as well either disease defining and/or clinically significant. Can include references in the table. For clinical significance, denote associations with FDA-approved therapy (not an extensive list of applicable drugs) and NCCN or other national guidelines if applicable; Can also refer to CGC workgroup tables as linked on the homepage if applicable as well as any high impact papers or reviews of gene mutations in this entity. Do not delete table.'')

+

{| class="wikitable sortable"

+

|-

+

!Gene; Genetic Alteration!!'''Presumed Mechanism (Tumor Suppressor Gene [TSG] / Oncogene / Other)'''!!'''Prevalence (COSMIC / TCGA / Other)'''!!'''Concomitant Mutations'''!!'''Mutually Exclusive Mutations'''

+

!'''Diagnostic Significance (Yes, No or Unknown)'''

+

!Prognostic Significance (Yes, No or Unknown)

+

!Therapeutic Significance (Yes, No or Unknown)

+

!Notes

+

|-

+

|EXAMPLE: ''TP53''; Variable LOF mutations

+

EXAMPLE:

−

*[[Primary Cutaneous CD30 Positive T-cell Lymphoproliferative Disorders]]

+

''EGFR''; Exon 20 mutations

−

~~- [[Lymphomatoid Papulosis]]~~

−

~~- [[Primary Cutaneous Anaplastic Large Cell Lymphoma]]~~

−

*[[Primary Cutaneous Peripheral T-~~cell Lymphomas, Rare Subtypes]]~~

+

EXAMPLE: ''BRAF''; Activating mutations

−

- ~~[[Primary Cutaneous Gamma Delta T~~-~~cell Lymphoma]]~~

+

|EXAMPLE: TSG

−

- ~~[[Primary Cutaneous CD8+ Aggressive Epidermotropic Cytotoxic T~~-~~cell Lymphoma]]~~

+

|EXAMPLE: 20% (COSMIC)

−

- ~~[[Primary Cutaneous Acral CD8+ T~~-~~cell Lymphoma]]~~

+

EXAMPLE: 30% (add Reference)

−

- ~~[[Primary Cutaneous CD4+ Small~~/~~Medium T~~-~~cell Lymphoproliferative Disorder]]~~

+

|EXAMPLE: ''IDH1'' R123H

+

|EXAMPLE: ''EGFR'' amplification

+

|EXAMPLE: Yes

+

|EXAMPLE: No

+

|EXAMPLE: No

+

|EXAMPLE:

−

*[~~[Peripheral T-cell Lymphoma~~, ~~Not Otherwise Specified~~ (~~NOS~~)]]

+

{| class="wikitable sortable"

+

|-

+

!Gene; Genetic Alteration!!'''Presumed Mechanism (Tumor Suppressor Gene [TSG] / Oncogene / Other)'''!!'''Prevalence (COSMIC / TCGA / Other)'''!!'''Concomitant Mutations'''!!'''Mutually Exclusive Mutations'''

+

!'''Diagnostic Significance (Yes, No or Unknown)'''

+

!Prognostic Significance (Yes, No or Unknown)

+

!Therapeutic Significance (Yes, No or Unknown)

+

!Notes

+

|-

+

|EXAMPLE: TP53; Variable LOF mutations

−

*[[Angioimmunoblastic T-~~cell Lymphoma and Other Nodal Lymphomas of T Follicular Helper Cell Origin]]~~

+

EXAMPLE:

−

~~- [[Angioimmunoblastic T-cell Lymphoma]]~~

−

~~- [[Follicular T-cell Lymphoma]]~~

−

~~- [[Nodal Peripheral T-cell Lymphoma with T Follicular Helper Phenotype]]~~

−

*[[Anaplastic Large Cell Lymphoma, ALK-Positive]]

+

EGFR; Exon 20 mutations

−

*[[Anaplastic Large Cell Lymphoma, ALK-~~Negative]]~~

+

EXAMPLE: BRAF; Activating mutations

+

|EXAMPLE: TSG

+

|EXAMPLE: 20% (COSMIC)

−

*[[Breast Implant-~~Associated Anaplastic Large Cell Lymphoma]]~~

+

EXAMPLE: 30% (add Reference)

+

|EXAMPLE: IDH1 R123H

+

|EXAMPLE: EGFR amplification

+

|

+

|

+

|

+

|EXAMPLE: Excludes hairy cell leukemia (HCL) (add reference).

+

+

|}

+

Note: A more extensive list of mutations can be found in cBioportal (https://www.cbioportal.org/), COSMIC (https://cancer.sanger.ac.uk/cosmic), ICGC (https://dcc.icgc.org/) and/or other databases. When applicable, gene-specific pages within the CCGA site directly link to pertinent external content.

−

<~~comments~~ />

+

<blockquote class='blockedit'>{{Box-round|title=v4:Gene Mutations (SNV/INDEL)|The content below was from the old template. Please incorporate above.}}

+

A few genes were noted to be altered during the transformed stages of CML, namely TP53'', RB1, MYC, CDKN2A, NRAS, KRAS, RUNX1, MECOM, TET2, CBL, ASXL1, IDH1'' and ''IDH2''.

+

</blockquote>

+

==Epigenomic Alterations==

+

Not Applicable.

+

==Genes and Main Pathways Involved==

+

Put your text here and fill in the table (''Instructions: Can include references in the table. Do not delete table.'')

+

{| class="wikitable sortable"

+

|-

+

!Gene; Genetic Alteration!!Pathway!!Pathophysiologic Outcome

+

|-

+

|EXAMPLE: ''BRAF'' and ''MAP2K1''; Activating mutations

+

|EXAMPLE: MAPK signaling

+

|EXAMPLE: Increased cell growth and proliferation

+

|-

+

|EXAMPLE: ''CDKN2A''; Inactivating mutations

+

|EXAMPLE: Cell cycle regulation

+

|EXAMPLE: Unregulated cell division

+

|-

+

|EXAMPLE: ''KMT2C'' and ''ARID1A''; Inactivating mutations

+

|EXAMPLE: Histone modification, chromatin remodeling

+

|EXAMPLE:

+

{| class="wikitable sortable"

+

|-

+

!Gene; Genetic Alteration!!Pathway!!Pathophysiologic Outcome

+

|-

+

|EXAMPLE: BRAF and MAP2K1; Activating mutations

+

|EXAMPLE: MAPK signaling

+

|EXAMPLE: Increased cell growth and proliferation

+

|-

+

|EXAMPLE: CDKN2A; Inactivating mutations

+

|EXAMPLE: Cell cycle regulation

+

|EXAMPLE: Unregulated cell division

+

|-

+

|EXAMPLE: KMT2C and ARID1A; Inactivating mutations

+

|EXAMPLE: Histone modification, chromatin remodeling

+

|EXAMPLE: Abnormal gene expression program

+

|}

+

<blockquote class='blockedit'>{{Box-round|title=v4:Genes and Main Pathways Involved|The content below was from the old template. Please incorporate above.}}

+

[[File:BCR-ABL-ASS1 abnormal double fusions.jpg|thumb|Image courtesy of Fabiola Quintero-Rivera, MD]]

+

Breakpoint Cluster Region protein (BCR) is encoded by ''BCR'' gene, located on chromosome 22. BCR protein has serine/threonine kinase activity.<ref name=":0" /> The protein is also a GTPase-activating protein for p21rac and other kinases.<ref>{{Cite journal|title=BCR BCR activator of RhoGEF and GTPase [Homo sapiens (human)] - Gene - NCBI|url=https://www.ncbi.nlm.nih.gov/gene?cmd=Retrieve&dopt=full_report&list_uids=613}}</ref> BCR protein is involved in the two main pathways: FGFR1 mutant receptor activation and G-protein signaling HRAS regulation pathway.<ref>{{Cite journal|last=Mn|first=Peiris|last2=F|first2=Li|last3=Dj|first3=Donoghue|date=2019|title=BCR: A Promiscuous Fusion Partner in Hematopoietic Disorders|url=https://pubmed.ncbi.nlm.nih.gov/31105873/|language=en|doi=10.18632/oncotarget.26837|pmc=PMC6505627|pmid=31105873}}</ref> BCR-associated genetic rearrangement gives rise to hematological disorders. The ''ABL1'' gene is located on chromosome 9q34.12 and encodes for ABL1 protein, which was discovered to be a tyrosine kinase protein.<ref>{{Cite journal|last=B|first=Chereda|last2=Jv|first2=Melo|date=2015|title=Natural Course and Biology of CML|url=https://pubmed.ncbi.nlm.nih.gov/25814077/|language=en|pmid=25814077}}</ref> Depending on the breakpoint of the ''BCR'' gene, the size of the fusion protein can vary: p190bcr-abl, p210bcr-abl, and p230bcr-abl, leading to three different isoforms.<ref name=":0" /> ''BCR-ABL1'' gene fusion encodes a chimeric protein, which is mostly 210 kDa(P210''BCRABL1'') with constitutive tyrosine-kinase activity, escaping the cytokine regulation and regulatory controls of many intracellular signaling pathways that are associated with proliferation, differentiation and apoptosis.<ref>{{Cite journal|last=Jb|first=Konopka|last2=Sm|first2=Watanabe|last3=On|first3=Witte|date=1984|title=An Alteration of the Human C-Abl Protein in K562 Leukemia Cells Unmasks Associated Tyrosine Kinase Activity|url=https://pubmed.ncbi.nlm.nih.gov/6204766/|language=en|pmid=6204766}}</ref><ref>{{Cite journal|last=R|first=Ren|date=2005|title=Mechanisms of BCR-ABL in the Pathogenesis of Chronic Myelogenous Leukaemia|url=https://pubmed.ncbi.nlm.nih.gov/15719031/|language=en|pmid=15719031}}</ref> Many of the target proteins that are affected by dimerization of constitutive kinase activity of BCR-ABL fusion protein include STAT, RAS, RAF, JUN kinase, MYC, AKT, and other transducers.<ref>{{Cite journal|last=S|first=Faderl|last2=M|first2=Talpaz|last3=Z|first3=Estrov|last4=S|first4=O'Brien|last5=R|first5=Kurzrock|last6=Hm|first6=Kantarjian|date=1999|title=The Biology of Chronic Myeloid Leukemia|url=https://pubmed.ncbi.nlm.nih.gov/10403855/|language=en|pmid=10403855}}</ref><ref>{{Cite journal|last=Cl|first=Sawyers|date=1999|title=Chronic Myeloid Leukemia|url=https://pubmed.ncbi.nlm.nih.gov/10219069/|language=en|pmid=10219069}}</ref> It was shown that when CML progresses to the blastic crisis phase, a new additional mutation is acquired GSK3beta, which leads to the activation of beta-catenin, preventing myeloid cell lineages to mature.<ref>{{Cite journal|last=Ch|first=Jamieson|last2=Le|first2=Ailles|last3=Sj|first3=Dylla|last4=M|first4=Muijtjens|last5=C|first5=Jones|last6=Jl|first6=Zehnder|last7=J|first7=Gotlib|last8=K|first8=Li|last9=Mg|first9=Manz|date=2004|title=Granulocyte-macrophage Progenitors as Candidate Leukemic Stem Cells in Blast-Crisis CML|url=https://pubmed.ncbi.nlm.nih.gov/15306667/|language=en|pmid=15306667}}</ref><ref>{{Cite journal|last=Ae|first=Abrahamsson|last2=I|first2=Geron|last3=J|first3=Gotlib|last4=Kh|first4=Dao|last5=Cf|first5=Barroga|last6=Ig|first6=Newton|last7=Fj|first7=Giles|last8=J|first8=Durocher|last9=Rs|first9=Creusot|date=2009|title=Glycogen Synthase Kinase 3beta Missplicing Contributes to Leukemia Stem Cell Generation|url=https://pubmed.ncbi.nlm.nih.gov/19237556/|language=en|doi=10.1073/pnas.0900189106|pmc=PMC2646624|pmid=19237556}}</ref>

+

[[File:9;22 image2K Abnormal Karyogram.jpg|thumb|Image courtesy of Fabiola Quintero-Rivera, MD]]

+

</blockquote>

+

==Genetic Diagnostic Testing Methods==

+

Majority of the patients with CML are initially diagnosed through a blood test - complete blood count - before clinical manifestations. Bone marrow aspirate and core biopsy are performed sequentially to further support the process of making diagnosis as well as assessing percentage of blasts and basophils.<ref>{{Cite journal|last=E|first=Jabbour|last2=H|first2=Kantarjian|date=2018|title=Chronic Myeloid Leukemia: 2018 Update on Diagnosis, Therapy and Monitoring|url=https://pubmed.ncbi.nlm.nih.gov/29411417/|language=en|pmid=29411417}}</ref> Histologic features of CML in the peripheral blood are helpful in deriving the CML diagnosis. Ancillary tests are performed to clinch the diagnosis: immunohistochemistry, flow cytometry, conventional cytogenetic analysis, FISH and molecular RT-PCR-based studies.

+

Cytogenetic testing is used in CML patients to monitor how patients are responding to the treatment by detecting the number of cells with the Philadelphia chromosome. In conjunction with cytogenetic testing, FISH and PCR are ordered to quantify treatment monitoring processes in CML. FISH allows the detection of ''BCR-ABL'' gene, which is essentially considered to be more of a sensitive test compared to cytogenetic testing. PCR is performed to find ''BCR-ABL'' fusion gene and other molecular abnormalities. PCR is very efficient because it can detect even one abnormal cell from approximately 1 million healthy cells. FISH can be used in rare cases where molecular transcripts are not detected.

+

Continuous monitoring is part of the standard of care in CML patients because it allows the clinicians to identify treatment failure, disease evolution and drug regimen adherence. Minimal residual disease monitoring is done by using RT-PCR. Major molecular response (MMR) is the critical goal of CML treatment. Complete or deep molecular response is achieved when there is absence of BCR-ABL1 transcript or >4.5 logs below baseline level.<ref>{{Cite journal|last=gknation|date=2015|title=Treatment Outcomes|url=https://www.lls.org/leukemia/chronic-myeloid-leukemia/treatment/treatment-outcomes|language=en}}</ref>

+

==Familial Forms==

+

Not Applicable.

+

==Additional Information==

+

Put your text here

+

==Links==

+

[[ABL1]]

+

[[BCR]]

+

==References==

+

(use the "Cite" icon at the top of the page) (''Instructions: Add each reference into the text above by clicking on where you want to insert the reference, selecting the “Cite” icon at the top of the page, and using the “Automatic” tab option to search such as by PMID to select the reference to insert. The reference list in this section will be automatically generated and sorted.'' ''If a PMID is not available, such as for a book, please use the “Cite” icon, select “Manual” and then “Basic Form”, and include the entire reference''''.'') <references />

+

'''

+

==Notes==

+

<nowiki>*</nowiki>Primary authors will typically be those that initially create and complete the content of a page. If a subsequent user modifies the content and feels the effort put forth is of high enough significance to warrant listing in the authorship section, please contact the CCGA coordinators (contact information provided on the homepage). Additional global feedback or concerns are also welcome.

+

<nowiki>*</nowiki>''Citation of this Page'': “Chronic myeloid leukaemia”. Compendium of Cancer Genome Aberrations (CCGA), Cancer Genomics Consortium (CGC), updated {{REVISIONMONTH}}/{{REVISIONDAY}}/{{REVISIONYEAR}}, <nowiki>https://ccga.io/index.php/HAEM5:Chronic_myeloid_leukaemia</nowiki>.

+

[[Category:HAEM5]][[Category:DISEASE]][[Category:Diseases C]]

Bailey.Glen

Autochecked users, Comment administrators, Editors, Interface administrators, Reviewers, Suppressors, Administrators, Widget editors

1,876

edits

Changes

Test (view source)

Revision as of 13:04, 1 May 2024