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Statistical, Computational, and Informatics Tools for Biomarker Analysis

Statistical, Computational, and Informatics Tools for Biomarker Analysis. Methodology Development at the D ata M anagement and C oordinating C enter of the E arly D etection R esearch N etwork. Early Detection Research Network. 18 Laboratories. 2 Laboratories NIST. 8 Centers

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Statistical, Computational, and Informatics Tools for Biomarker Analysis

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  1. Statistical, Computational, and Informatics Tools for Biomarker Analysis Methodology Development at the Data Management and Coordinating Center of the Early Detection Research Network

  2. Early Detection Research Network 18 Laboratories 2 Laboratories NIST 8 Centers CDCP Chair: Bernard Levin Chair: David Sidransky EDRN ORGANIZATIONAL STRUCTURE An “infrastructure” for supporting collaborative research on molecular, genetic and other biomarkers in human cancer detection and risk assessment.

  3. Early Detection Research Network INFRASTRUCTURE BIOREPOSITORY • Specimens with matching controls and • epidemiological data • Infrastructure to provide preneoplastic tissues: • - Prostate • - Lung • - Ovarian • - Colon • - Breast

  4. Early Detection Research Network INFRASTRUCTURE LABORATORY CAPACITY • Capability in high-throughput molecular and biochemical assays • Ability to respond to evolving technologies for EDRN needs • Extensive experience and scale-up ability in proteomics and • molecular assays • Outstanding infrastructure for handling multiple assays and • validation requests

  5. Early Detection Research Network INFRASTRUCTURE DATA STORAGE AND MINING • Outstanding track record in biomarker research • Statistical and data mining technology • Statistical and predictive models for multiple biomarkers • Novel statistical methods to interpret high-throughput data

  6. Early Detection Research Network INFRASTRUCTURE DATA EXCHANGE AND SHARING • Improving informatics and information flow • Network web sites • public web site • secure web site • Early Detection Research Network Exchange (ERNE) • Standardizing of Data Reporting: CDEs Developed

  7. Early Detection Research Network (EDRN) INFORMATICS AND INFORMATION FLOW

  8. EARLY DETECTION RESEARCH NETWORK COLLABORATION How To Become an Associate Member • Contact one of the EDRN Principal Investigators to serve as a sponsor for an application. Three types of collaborative opportunities are available: • Type A: Novel research ideas complementing EDRN ongoing efforts; one year of funding at $100,000 • Type B: Share tools, technology and resources, no time limit • Type C: Allow to participate in the EDRN Meetings and Workshop • For details on how to apply, see http://www.cancer.gov/edrn

  9. DMCC Statisticians • Margaret Pepe, Lead of Methodology Group • Ziding Feng, Principal Investigator • Yinsheng Qu • Mary Lou Thompson • Mark Thornquist • Yutaka Yasui

  10. Biomarker Lab Collaborators at Eastern Virginia Medical School • Bao-Ling Adam • John Semmes • George Wright

  11. Focus of Presentation • Design:Phase Structure for Biomarker Research • Analysis:Statistical Methods for Biomarker Discovery from High-Dimensional Data Sets

  12. Design: Phase Structure for Biomarker Research Three phase structure for therapeutic trials well-established Structure promotes coherent, thorough, efficient development Similar structure needs to be developed for biomarker research

  13. Biomarker Development • Categorize process into 5 phases • Define objectives for each phase • Define ideal study designs, evaluation and criteria for proceeding further • Standardize the process to promote efficiency and rigor

  14. The Details of Study Design • Specific Aims • Subject/Specimen Selection • Outcome measures • Evaluation of Results • Sample Size Calculations • Limitations / Pitfalls

  15. Phase 1 Identify leads for potentially useful biomarkers Prioritize these leads Phase 2 Determine the sensitivity and specificity or ROC curve for the clinical biomarker assay in discriminating clinical cancer from controls Specific Aims

  16. Phase 1 Cancers that are ultimately serious if not treated early, but treatable in early stage Spectrum of sub-types Collected at diagnosis Phase 2: same criteria as for phase 1 Wide spectrum of cases Clinical specimen at diagnosis From target screening population Specimen Selection -- Cases

  17. Phase 1 Non-cancer tissue same organ same patient Normal tissue non-cancer patient Benign growth tissue non-cancer patient Phase 2 From potential target population for screening Specimen Selection -- Controls

  18. Phase 1 True positive and False positive rates (binary result) True positive rate at threshold yielding acceptable false positive rate ROC curve Phase 2 Results of clinical biomarker assay Outcome Measures

  19. Phase 1 Algorithms select and prioritize markers that best distinguish tumor from non-tumor tissue Initial exploratory studies need confirmation with new validation specimens Phase 2 ROC curves ROC regression to determine if characteristics of cases and/or characteristics of controls effect biomarker’s discriminatory capacity Evaluation of Results

  20. Phase 1 Should be large enough so that very promising biomarkers are likely to be selected for phase 2 development Phase 2 Based on a confidence intervals for the TPR or FPR, or confidence intervals for the ROC curve at selected critical points Sample Size

  21. Findings: Sample Size Estimation • For phase 1 microarray experiments, use of ROC curves is more efficient than comparing means • For phase 2 studies, equal numbers of cases and controls is often not optimally efficient • Sample size calculations and look-up tables are now in EDRN website

  22. Pepe et al. Phases of biomarker development for early detection of cancer. Journal of the National Cancer Institute 93(14):1054–61, 2001. Pepe et al. “Elements of Study Design for Biomarker Development” InTumor Markers, Diamandis, Fritsche, Lilja, Chan, and Schwartz , eds. AAAC Press, Washington, DC. 2002. 3. Pepe. “Statistical Evaluation of Diagnostic Tests & Biomarkers” Oxford U. Press, 2003.

  23. Selecting Differentially Expressed Genes from Microarray ExperimentsLead: Margaret Pepe • Context • gene expression arrays for nD tumor tissues and nCnormal tissues • Yig = logarithm relative intensity at gene g for tissue i. • for which genes are Yig different in some/most cases from the normals? • how many tissues, nD andnC,should be evaluated in these experiments? • illustrated with ovarian cancer data

  24. Statistical Measures for Gene Selection — typically use a two sample t-test for each gene — we argue that sensitivity and specificity are more directly relevant for cancer biomarker research. — focus attention on high specificity (or high sensitivity) — use the partial area under the ROC curve to rank genes, instead of the t-test

  25. Example

  26. Sample Sizes for Gene Discovery Studies • traditional calculations based on statistical hypothesis testing • These are exploratory studies, need new methods • Propose to base calculations on the probability that a differentially expressed gene will rank high among all genes • Use computer simulation for sample size calculations

  27. with 50 tumor and 50 normal tissues we can be 83.6% sure that the top 30 genes will rank in the top 100 in the experiment.

  28. Pepe et al. Selecting differentially expressed genes from microarray experiments. Biometrics (in press)

  29. Summary • The method we developed for selecting genes and calculating sample sizes are more appropriate for the purpose of diagnosis and early detection

  30. Analysis:Statistical Methods for Biomarker Discovery from High-Dimensional Data Sets • Method development motivated by SELDI data from John Semmes/George Wright at Eastern Virginia Medical School • Data consist of protein intensities at tens of thousands of mass/charge points on each of 297 individuals • Developed three approaches to biomarker discovery: wavelets, boosting decision tree, and automated peak identification

  31. The EVMS prostate cancer biomarker project • Prostate cancer patients: N=99 early-stage N=98 late-stage • Normal controls N=96 • Serum samples for proteomic analysis by Surface Enhanced Laser Desorption/Ionization (SELDI) • Goal: To discover protein signals that distinguish cancers from normals

  32. An example of SELDI output 48,000 mass/charge points (200K Da)

  33. Test Data Training Data 30 PCa 15 Normal (Blinded) 167 PCa (84 early, 83 late) vs. 81 Normal The design of the biomarker analysis Normal PCa-early PCa-late N=96 N=99 N=98

  34. Wavelet AnalysisLead: Yinsheng Qu Steps in the wavelet analysis: • Represent original data plot with a set of wavelets (dimension reduction) • Determine those wavelets that distinguish between subgroups (information criterion) • Define discriminating functions based on the distinguishing wavelets (Fisher discrimination)

  35. Three Group Classification:Normal, Cancer, BPH 12,352 mass spectrum data points, reduced to 3,420 Haar wavelet coefficients, of which 17 coefficients distinguish between the three cases. 2 classification functions generated. Truth: Predicted: Normal Cancer BPH Normal 14 0 0 Cancer 1 27 7 BPH 0 3 8

  36. Qu Y et al. Data reduction using discrete wavelet transform in discriminant analysis with very high dimension. Biometrics, in press.

  37. Boosted Decision Tree Method. Lead: Yinsheng Qu/Yutaka Yasui • This method combines multiple weak learners into a very accurate classifier • It can be used in cancer detection • It can also be used in identification of tumor markers • Using this method we can separate controls, BPH, and PCA without error in test set

  38. Outline of boosting decision tree • The combined classifier is a committee with the decision stumps, the base classifiers, as its members. It makes decisions by majority vote. • The base classifiers are constructed on weighted examples: the examples misclassified will increase their weights on next round. • The 2nd stump’s specialty is to correct the 1st stump’s mistakes, and the 3rd stump’s specialty is to correct the 2nd stump’s mistakes, and so on. • The combined classifier with dozens and even hundreds of decision stumps will be accurate. • Boosting technique is resistant to over fitting.

  39. Classifier 2: A boosted decision stump classifier with 21 peaks (potential markers)

  40. The Boosting procedure • Yi={cancer, normal}={1, -1}, fm(xi)={1, -1} • Initial weights (m=1), wi = 1 (i = 1, . . .,N). • Choose first peak and threshold c. • For m =1 to M: wi = wi exp{amI(incorrect)} • where am = ln(1-err)/err) and err is the classification error rate at the current stage • normalize the weights so they sum to N. • choose a peak and c (i-th subject with weight wi) • Final classifier: f(x) = sum(amfm(x)) over m=1 to M. f(xi)> 0  i-th subject classified as cancer

  41. When to stop iteration? • minimal margin: minimum of yi f(xi) over all N subjects • The minimal margin in the training sample measures how well the two classes are separated by classifier. • Even classifier reaches zero error on training sample, if iteration still increases the minimal margin --> improve prediction in future samples.

  42. Qu et al. 2002. Boosted Decision Tree Analysis of SELDI Mass Spectral Serum Profiles Discriminates Prostate Cancer from Non-Cancer Patients. Clinical Chemistry. In press. Adam et al. 2002. Serum Protein Fingerprinting Coupled with a Pattern Matching Algorithm that Distinguishes Prostate Cancer from Benign Prostate Hyperplasia and Healthy Men. Cancer Research. 62:3609-3614.

  43. Summary • Wavelets approach: Does not require peak identification (black-box classification) • Boosting decision tree: Requires peak identification first. Useful for both classification and protein mass identification

  44. Final Summary • The methods developed in the past two years are mainly for Phase 1&2 studies, reflecting the current needs of EDRN. • EDRN DMCC statisticians are working on key design and analysis issues in early detection research. • More work remains to be done (e.g., In classification, consider the mislabeling of Prostate cancer by BPH; exam gene by environmental interactions).

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