CLL Sample! Clinical Trials! Accrual, tracking,! correlative studies! Immunophenotyping! Surface & intracellular! ZAP-70/CD38! prognosis!

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ZAP-70/CD38! prognosis! IGHV! Mutational status! prognosis! Cytogenetics! FISH! karyotype! Cellular Kinetics! B-cell turnover rates! CD38/Ki67/CXCR4! Buccal swabbs! Germline DNA! Genetics studies! Immunophenotyping! Surface & intracellular! CLL Sample! (N = 5,300)! Demographic! Age, sex, race! Clinical Trials! Accrual, tracking,! correlative studies! Clinical data! WBC,Rai,! Dx, Tx! Serial samples! Longitudinal studies! DNA& RNA! Molecular studies! Plasma/Serum! ELISAs! Blood smears! Immunohistochemistry!

1) Immunophenotyping : ZAP studies, others markers :Ki67, CXCR4, TCL-1 2) IGHV mutation status : VH studies 3) Cytogenetics : QA/QC, Cyto studies 4) Clinical : data entry, QA/QC CRC Clinical trials 5) CRC Clinical trials: facilitate correlative science 6) Serial samples : Longitudinal studies, disease evolution

Stain # FL1 (FITC) FL2 (PE) FL3 (PerCP) FL4 ( APC) 1 Iso1 Iso1 Iso1 Iso1 2 Ki67 CD38 CD19 TCL-1 3 Ki67 CD5 CD19 CXCR4 4 ZAP CD3 CD19 CD5 5 lambda kappa CD20 CD19 6 CD23 CD38 CD19 CD5 7 IgM IgD CD19 4A5

2100/5300 (40%) pts in CRC have serial samples *N=200 to *N=2100 ------>10 fold increase serial sample accrual SUM accrual Pts with serial samples 2500 2000 * 1500 1000 500 0 Dec 02 * Dec 03 Dec 04 Dec 05 Dec 06 Dec 07 Dec 08 Dec 09 Dec 10

A = pt has non-progressive disease & stable WBC over time B = pt has exponential increase in WBC over time C = pt has an acceleration in the kinetics of the leukemia cell doubling time Merit: Longitudinal studies Acquisition of serial samples enables studies on the different kinetics in the increase of WBC over time. Review of the clinical data on all these cases characterized by serial samples, will allow the CRC investigators to segregate cases that have indolent & non-progressive disease from those who have a change in the kinetics of disease progression (core A & B).

Sample Evaluator (%) ALL CRC Sites 1/5/2010 Sample Evaluator (%) ALL CRC Sites 1/4/2011 A B C D F A B C D F A pts= serial smpls : at least 3 smpls & clinical data on at least 2 smpls B pts= serial smpls : at least 2 smpls & clinical data on at least 1 smpl C pst = one sample : 1 & clinical data on 1 smpl D pts = one sample : clinical data not yet present

Tissue Core - FISH studies Cytogenetics Team! CRC Cytogenetics Lab Directors: Daniel Van Dyke Mayo Clinic Nyla Heerema Ohio State University Paola Dal Cin Brigham and Women's Hospital(DF) Marie Dell'Aquila UC San Diego Ayala Aviram Long Island Jewish CRC Coordinators/Interactions: Laura Rassenti Coordinate(UCSD) ------>studies/data updates Andrew Greaves Data (UCSD)----->input/storage/output Donna Neuberg Biostats (DF)---->oversee data/studies design Jeanette Eckel-Passow Biostats Mayo----> QA/QC data (SAS) Carlo Croce Project 1(OSU)------>use of data/collaborations All CRC PIs for Clinical data updates, FISH data -----> mining/studies ***Monthly teleconferences ***CRC FISH website (all updates) https://cllresearch3.ucsd.edu/!

Role of CRC Cytogeneticists 1) Oversee FISH & karyotype uniform data entry from CRC Sites Data entered for each sample with blood in the Tissue Core: close to DX, serials, before 1st Tx 2) Assure QA/QC of all FISH Data for data retreival by CRC Mayo : Jeanette Eckel Passow DF: Donna 3) Individual Cytogeneticist Hypothesis-driven study

Tissue Core Cytogeneticists accomplishments: 2 publications! Heerema et all. Chronic Lymphocytic Leukemia Research Consortium. Stimulation of chronic lymphocytic leukemia cells with CpG oligodeoxynucleotide gives consistent karyotypic results among laboratories: a CLL Research Consortium (CRC) Study. Cancer Genet Cytogenet. 2010 Dec;203(2):134-40. Smoley et al. Standardization of fluorescence in situ hybridization studies on chronic lymphocytic leukemia (CLL) blood and marrow cells by the CRC. Cancer Genet Cytogenet. 2010 Dec;203(2):141-8.

Tissue Core FISH studies Data accrual Update! Standarized FISH scoring, data entry, & retrieval *Dec 1, 05 = 15% of CRC pts had FISH data *Dec 1, 10 = 62 % of CRC pts have FISH data 5 Fold Increase in FISH Data Accrual % of CRC pts with FISH data 3300/5300 (62%) % 100 80 60 40 20 * * 0 Dec 04 Dec 05 Dec 06 Dec 07 Dec 08 Dec 09 Dec 10

Tissue Core Cellular Kinetics/IGHV studies Presentation by : Nicholas Chiorazzi, MD Professor of Medicine and Cell Biology,Albert Einstein College of Medicine Investigator, The Feinstein Institute for Medical Research North Shore-Long island Jewish Health Systems, NY 1) Cellular Kinetics: use of Tissue Core immunophenotyping data A) Surface 4-color-Immunophenotyping : to date CLLs characterized N=4,600 (90%) CD5/CD19/Kappa/Lambda/CD3/CD23/CD20/CD38/ROR1/CXCR4 B) Intracellular immunophenotyping : to date CLLs characterized N=4,600(90%) ZAP-70, TCL1, Ki67 All data analyzed by Flow-Jo software & entered in the CRC database Correlations with prognostic markers/serial samples/longitudinal studies 2) IGHV studies : use of Tissue Core IGHV mutational status data IGHV mutation status : to date CLLs characterized N= 3,300 (65%) all sequence data analyzed by: IMGT/V-Quest :http:/imgt.cines.fr/imgt_vquest all data uniformly entered & retrieved All Interactions with informatics & biostatistics (Cores A & B)

Use of acquired data: Cores A,B,D All Projects Chiorazzi/Kipps : VH studies, CLL antigens B cell proliferation compartment Croce: TCL1 studies Kipps: role ROR1, NLC Kay/Burger: NLC - stroma Byrd: methylation Merit: 1) Prognosis/Therapy 2) Clinical Trials: Correlative sciences Response to Tx 3) Longitudinal studies /Disease Evolution 4) Stability of markers over time

The Tissue Core acquires SERIAL samples during the disease progression of the CLL patients that are registered in the CRC. The serial samples of from the CLL patients are characterized according to their surface antigen phenotype by multiparameter flow cytometric analysis and clinical information. This enables the CRC investigators to examine for longitudinal changes in the leukemia cell's genotype, biochemistry, and/or immunologic phenotype and correlate these data to clinical outcome.

Use of acquired data: Cores A,B,D All Projects Chiorazzi/Kipps : B cell proliferation compartment Croce: TCL1/miRNA serial studies Kipps: role ROR1, NLC Kay/Burger: NLC - stroma Byrd: methylation Merit: 1) Prognosis/Therapy 2) Clinical Trials: Correlative sciences Response to Tx 3) Longitudinal studies /Disease Evolution 4) Stability of markers over time

Collection Schema Dx! Every 6 mo pretx Tx! Post Tx according to CRC protocols Core D 1! 2! 3! 4! Sample Collection: Blood (1,2,3,4) Buccal swabb (1) Plasma (1,2,3,4) Serum (1,2,3,4) Slides (1,2,3,4) Familial CLL smpls Use of Data: Cores A,B,D All Projects Merit of continued accrual: 1) Prognosis/Therapy 2) Correlative science 3) Longitudinal studies 4) Increase probability to capture pts with unique mutations (P1) Tissue Core : Monthly Updates of Samples Acquired & Distributed to all CRC members emails & Website : https://cllresearch3.ucsd.edu/ CLL Dx according to NCI 1996-revised guidelines Hallek et al Blood 2008 (111):5446.

Chateau Lafite Rothschild - (yr 1959 @ $2,200/bottle) The CRC Tissue Core : Is getting better with time Thanks to all CRC members!

CRC Meeting ASH 2010 Thanks to all