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Your search keyword '"Greenbaum, Carla J."' showing total 5 results
Start Over Author "Greenbaum, Carla J." Journal plos one
5 results on '"Greenbaum, Carla J."'

1. Sensitive detection of multiple islet autoantibodies in type 1 diabetes using small sample volumes by agglutination-PCR.

Author

Cortez, Felipe de Jesus, Gebhart, David, Robinson, Peter V, Seftel, David, Pourmandi, Narges, Owyoung, Jordan, Bertozzi, Carolyn R, Wilson, Darrell M, Maahs, David M, Buckingham, Bruce A, Mills, John R, Roforth, Matthew M, Pittock, Sean J, McKeon, Andrew, Page, Kara, Wolf, Wendy A, Sanda, Srinath, Speake, Cate, Greenbaum, Carla J, and Tsai, Cheng-Ting

Subjects
Islets of Langerhans, Humans, Diabetes Mellitus, Type 1, Glutamate Decarboxylase, Autoantibodies, Insulin Antibodies, Mass Screening, Sensitivity and Specificity, Polymerase Chain Reaction, Agglutination, Adolescent, Adult, Female, Male, Young Adult, Diabetes Mellitus, Type 1, General Science & Technology
Abstract

Islet autoantibodies are predominantly measured by radioassay to facilitate risk assessment and diagnosis of type 1 diabetes. However, the reliance on radioactive components, large sample volumes and limited throughput renders radioassay testing costly and challenging. We developed a multiplex analysis platform based on antibody detection by agglutination-PCR (ADAP) for the sample-sparing measurement of GAD, IA-2 and insulin autoantibodies/antibodies in 1 μL serum. The assay was developed and validated in 7 distinct cohorts (n = 858) with the majority of the cohorts blinded prior to analysis. Measurements from the ADAP assay were compared to radioassay to determine correlation, concordance, agreement, clinical sensitivity and specificity. The average overall agreement between ADAP and radioassay was above 91%. The average clinical sensitivity and specificity were 96% and 97%. In the IASP 2018 workshop, ADAP achieved the highest sensitivity of all assays tested at 95% specificity (AS95) rating for GAD and IA-2 autoantibodies and top-tier performance for insulin autoantibodies. Furthermore, ADAP correctly identified 95% high-risk individuals with two or more autoantibodies by radioassay amongst 39 relatives of T1D patients tested. In conclusion, the new ADAP assay can reliably detect the three cardinal islet autoantibodies/antibodies in 1μL serum with high sensitivity. This novel assay may improve pediatric testing compliance and facilitate easier community-wide screening for islet autoantibodies.

Published
2020

2. Sensitive detection of multiple islet autoantibodies in type 1 diabetes using small sample volumes by agglutination-PCR

Author

de Jesus Cortez, Felipe, Gebhart, David, Robinson, Peter V, Seftel, David, Pourmandi, Narges, Owyoung, Jordan, Bertozzi, Carolyn R, Wilson, Darrell M, Maahs, David M, Buckingham, Bruce A, Mills, John R, Roforth, Matthew M, Pittock, Sean J, McKeon, Andrew, Page, Kara, Wolf, Wendy A, Sanda, Srinath, Speake, Cate, Greenbaum, Carla J, and Tsai, Cheng-ting

Subjects
Diabetes, Autoimmune Disease, Pediatric, 4.2 Evaluation of markers and technologies, 4.1 Discovery and preclinical testing of markers and technologies, Detection, screening and diagnosis, Metabolic and endocrine, Adolescent, Adult, Agglutination, Autoantibodies, Diabetes Mellitus, Type 1, Female, Glutamate Decarboxylase, Humans, Insulin Antibodies, Islets of Langerhans, Male, Mass Screening, Polymerase Chain Reaction, Sensitivity and Specificity, Young Adult, General Science & Technology
Abstract

Islet autoantibodies are predominantly measured by radioassay to facilitate risk assessment and diagnosis of type 1 diabetes. However, the reliance on radioactive components, large sample volumes and limited throughput renders radioassay testing costly and challenging. We developed a multiplex analysis platform based on antibody detection by agglutination-PCR (ADAP) for the sample-sparing measurement of GAD, IA-2 and insulin autoantibodies/antibodies in 1 μL serum. The assay was developed and validated in 7 distinct cohorts (n = 858) with the majority of the cohorts blinded prior to analysis. Measurements from the ADAP assay were compared to radioassay to determine correlation, concordance, agreement, clinical sensitivity and specificity. The average overall agreement between ADAP and radioassay was above 91%. The average clinical sensitivity and specificity were 96% and 97%. In the IASP 2018 workshop, ADAP achieved the highest sensitivity of all assays tested at 95% specificity (AS95) rating for GAD and IA-2 autoantibodies and top-tier performance for insulin autoantibodies. Furthermore, ADAP correctly identified 95% high-risk individuals with two or more autoantibodies by radioassay amongst 39 relatives of T1D patients tested. In conclusion, the new ADAP assay can reliably detect the three cardinal islet autoantibodies/antibodies in 1μL serum with high sensitivity. This novel assay may improve pediatric testing compliance and facilitate easier community-wide screening for islet autoantibodies.

Published
2020

4. Avidity-dependent programming of autoreactive T cells in T1D.

Author

Durinovic-Belló, Ivana, Gersuk, Vivian H, Ni, Chester, Wu, Rebecca, Thorpe, Jerill, Jospe, Nicholas, Sanda, Srinath, Greenbaum, Carla J, and Nepom, Gerald T

Subjects
T-Lymphocyte Subsets, Humans, Diabetes Mellitus, Type 1, Insulin, Proinsulin, Receptors, Antigen, T-Cell, Autoantigens, Case-Control Studies, Gene Expression Profiling, Autoimmunity, T-Cell Antigen Receptor Specificity, Protein Binding, Genotype, Adult, Middle Aged, Female, Male, Young Adult, Diabetes, Autoimmune Disease, Genetics, Underpinning research, 1.1 Normal biological development and functioning, Metabolic and endocrine, General Science & Technology
Abstract

Fate determination for autoreactive T cells relies on a series of avidity-dependent interactions during T cell selection, represented by two general types of signals, one based on antigen expression and density during T cell development, and one based on genes that interpret the avidity of TCR interaction to guide developmental outcome. We used proinsulin-specific HLA class II tetramers to purify and determine transcriptional signatures for autoreactive T cells under differential selection in type 1 diabetes (T1D), in which insulin (INS) genotypes consist of protective and susceptible alleles that regulate the level of proinsulin expression in the thymus. Upregulation of steroid nuclear receptor family 4A (NR4A) and early growth response family genes in proinsulin-specific T cells was observed in individuals with susceptible INS-VNTR genotypes, suggesting a mechanism for avidity-dependent fate determination of the T cell repertoire in T1D. The NR4A genes act as translators of TCR signal strength that guide central and peripheral T cell fate decisions through transcriptional modification. We propose that maintenance of an NR4A-guided program in low avidity autoreactive T cells in T1D reflects their prior developmental experience influenced by proinsulin expression, identifying a pathway permissive for autoimmunity.

Published
2014

5. Sample Size Requirements for Studies of Treatment Effects on Beta-Cell Function in Newly Diagnosed Type 1 Diabetes.

Author

Lachin, John M., McGee, Paula L., Greenbaum, Carla J., Palmer, Jerry, Pescovitz, Mark D., Gottlieb, Peter, and Skyler, Jay

Subjects
PANCREATIC beta cells, TYPE 1 diabetes, PEPTIDES, MEDICAL research, MEDICAL sciences
Abstract

Preservation of β-cell function as measured by stimulated C-peptide has recently been accepted as a therapeutic target for subjects with newly diagnosed type 1 diabetes. In recently completed studies conducted by the Type 1 Diabetes Trial Network (TrialNet), repeated 2-hour Mixed Meal Tolerance Tests (MMTT) were obtained for up to 24 months from 156 subjects with up to 3 months duration of type 1 diabetes at the time of study enrollment. These data provide the information needed to more accurately determine the sample size needed for future studies of the effects of new agents on the 2-hour area under the curve (AUC) of the C-peptide values. The natural log(x), log(x+1) and square-root (√x ) transformations of the AUC were assessed. In general, a transformation of the data is needed to better satisfy the normality assumptions for commonly used statistical tests. Statistical analysis of the raw and transformed data are provided to estimate the mean levels over time and the residual variation in untreated subjects that allow sample size calculations for future studies at either 12 or 24 months of follow-up and among children 8-12 years of age, adolescents (13-17 years) and adults (18+ years). The sample size needed to detect a given relative (percentage) difference with treatment versus control is greater at 24 months than at 12 months of follow-up, and differs among age categories. Owing to greater residual variation among those 13-17 years of age, a larger sample size is required for this age group. Methods are also described for assessment of sample size for mixtures of subjects among the age categories. Statistical expressions are presented for the presentation of analyses of log(x+1) and √x transformed values in terms of the original units of measurement (pmol/ml). Analyses using different transformations are described for the TrialNet study of masked anti-CD20 (rituximab) versus masked placebo. These results provide the information needed to accurately evaluate the sample size for studies of new agents to preserve C-peptide levels in newly diagnosed type 1 diabetes. [ABSTRACT FROM AUTHOR]

Published
2011
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