A Plasma-Based Protein Marker Panel for Colorectal Cancer Detection Identified by Multiplex Targeted Mass Spectrometry

被引:28
|
作者
Jones, Jeffrey J. [1 ]
Wilcox, Bruce E. [1 ]
Benz, Ryan W. [1 ]
Babbar, Naveen [1 ]
Boragine, Genna [1 ]
Burrell, Ted [1 ]
Christie, Ellen B. [1 ]
Croner, Lisa J. [1 ]
Cun, Phong [1 ]
Dillon, Roslyn [1 ]
Kairs, Stefanie N. [1 ]
Kao, Athit [1 ]
Preston, Ryan [1 ]
Schreckengaust, Scott R. [1 ]
Skor, Heather [1 ]
Smith, William F. [1 ]
You, Jia [1 ]
Hillis, W. Daniel [2 ]
Agus, David B. [3 ,4 ]
Blume, John E. [1 ]
机构
[1] Appl Prote Inc, 3545 John Hopkins Court,Suite 150, San Diego, CA 92121 USA
[2] Appl Minds, Glendale, CA USA
[3] USC Norris Westside Canc Ctr, Beverly Hills, CA USA
[4] USC Ctr Appl Mol Med, Beverly Hills, CA USA
关键词
Classification; Colorectal cancer; Machine learning; Mass spectrometry; Multiple reaction monitoring; PEPTIDES; POLYPECTOMY; COLONOSCOPY; BIOMARKERS; PROTEOMICS; ASSAYS; TESTS; BLOOD; FIT;
D O I
10.1016/j.clcc.2016.02.004
中图分类号
R73 [肿瘤学];
学科分类号
100214 ;
摘要
Combining potential diagnostics markers might be necessary to achieve sufficient diagnostic test performance in a complex state such as cancer. Applying this philosophy, we have identified a 13-protein, blood-based classifier for the detection of colorectal cancer. Using mass spectrometry, we evaluated 187 proteins in a case-control study design with 274 samples and achieved a validation of 0.91 receiver operating characteristic area under the curve. Introduction: Colorectal cancer (CRC) testing programs reduce mortality; however, approximately 40% of the recommended population who should undergo CRC testing does not. Early colon cancer detection in patient populations ineligible for testing, such as the elderly or those with significant comorbidities, could have clinical benefit. Despite many attempts to identify individual protein markers of this disease, little progress has been made. Targeted mass spectrometry, using multiple reaction monitoring (MRM) technology, enables the simultaneous assessment of groups of candidates for improved detection performance. Materials and Methods: A multiplex assay was developed for 187 candidate marker proteins, using 337 peptides monitored through 674 simultaneously measured MRM transitions in a 30-minute liquid chromatography-mass spectrometry analysis of immunodepleted blood plasma. To evaluate the combined candidate marker performance, the present study used 274 individual patient blood plasma samples, 137 with biopsy-confirmed colorectal cancer and 137 age-and gender-matched controls. Using 2 well-matched platforms running 5 days each week, all 274 samples were analyzed in 52 days. Results: Using one half of the data as a discovery set (69 disease cases and 69 control cases), the elastic net feature selection and random forest classifier assembly were used in cross-validation to identify a 15-transition classifier. The mean training receiver operating characteristic area under the curve was 0.82. After final classifier assembly using the entire discovery set, the 136-sample (68 disease cases and 68 control cases) validation set was evaluated. The validation area under the curve was 0.91. At the point of maximum accuracy (84%), the sensitivity was 87% and the specificity was 81%. Conclusion: These results have demonstrated the ability of simultaneous assessment of candidate marker proteins using high-multiplex, targeted-mass spectrometry to identify a subset group of CRC markers with significant and meaningful performance.
引用
收藏
页码:186 / +
页数:22
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