Your search keyword '"Preffer F"' showing total 21 results

1. Optimization of a flow cytometry test for routine monitoring of B cell maturation antigen targeted CAR in peripheral blood.

Author

Lee WH, Graham CE, Wiggin HR, Nolan HK, Graham KJ, Korell F, Leick MB, Barselau AL, Emmanuel-Alejandro E, Trailor MA, Gildea JM, Preffer F, Frigault MJ, Maus MV, and Gallagher KME

Subjects

Humans, T-Lymphocytes immunology, Flow Cytometry methods, B-Cell Maturation Antigen immunology, Receptors, Chimeric Antigen immunology, Immunotherapy, Adoptive methods, Multiple Myeloma immunology, Multiple Myeloma diagnosis, Multiple Myeloma blood

Abstract

Chimeric antigen receptor (CAR) modified T cell therapies targeting BCMA have displayed impressive activity in the treatment of multiple myeloma. There are currently two FDA licensed products, ciltacabtagene autoleucel and idecabtagene vicleucel, for treating relapsed and refractory disease. Although correlative analyses performed by product manufacturers have been reported in clinical trials, there are limited options for reliable BCMA CAR T detection assays for physicians and researchers looking to explore it as a biomarker for clinical outcome. Given the known association of CAR T cell expansion kinetics with toxicity and response, being able to quantify BCMA CAR T cells routinely and accurately in the blood of patients can serve as a valuable asset. Here, we optimized an accurate and sensitive flow cytometry test using a PE-conjugated soluble BCMA protein, with a lower limit of quantitation of 0.19% of CD3+ T cells, suitable for use as a routine assay for monitoring the frequency of BCMA CAR T cells in the blood of patients receiving either ciltacabtagene autoleucel or idecabtagene vicleucel., (© 2024 International Clinical Cytometry Society.)

Published

2024

2. Noel Warner Ph.D.

Author

Preffer F, Dunne J, Recktenwald D, Blidy A, Lanier L, Trotter J, and Daley MJ

Subjects

Humans, Flow Cytometry

Published

2023

3. Editor's response to Bunting et al.

Author

Preffer F

Subjects

Humans, Flow Cytometry

Published

2021

4. Special Issue: Updated ICCS/ESCCA PNH guidelines.

Author

Preffer F

Subjects

Humans, Flow Cytometry methods

Published

2018

5. Utility of Flow Cytometry in Diagnosing Hematologic Malignancy in Tonsillar Tissue.

Author

Aisagbonhi O, DeLelys M, Hartford N, Preffer F, and Ly A

Subjects

Adolescent, Adult, Aged, Aged, 80 and over, Biopsy, Child, Child, Preschool, Female, Flow Cytometry economics, Frozen Sections, Hematologic Neoplasms surgery, Humans, Immunohistochemistry, Male, Middle Aged, Palatine Tonsil surgery, Rare Diseases surgery, Retrospective Studies, Tonsillar Neoplasms surgery, Tonsillectomy, Young Adult, Flow Cytometry statistics & numerical data, Hematologic Neoplasms pathology, Palatine Tonsil pathology, Rare Diseases pathology, Tonsillar Neoplasms pathology

Abstract

Objective: Tonsil surgical biopsy or excision is a very common procedure. However, there exist no consensus guidelines for the pathologic handling of tonsil specimens; gross and/or microscopic evaluation may be used. Diagnosis of tonsillar hematologic malignancy requires histology, immunohistochemistry and/or flow cytometry. Data regarding the utility of flow cytometry in tonsillar tissues are limited. We assessed our experience with flow cytometry for tonsil diagnosis with regard to accuracy and use patterns at a tertiary academic medical center., Methods: We retrospectively analyzed all surgically biopsied or excised tonsil specimens that underwent flow cytometry evaluation from August 2011 to March 2014. Patient clinical information, intraoperative frozen section, histology, immunohistochemistry, and flow cytometry diagnoses were recorded., Results: The study included 154 tonsil specimens from 89 females and 65 males. Patients averaged 27.4 years old (range 2-87 years); 73 were pediatric. Both histology and flow cytometry were benign for 148 patients (96.1%). Hematolymphoid malignancy was diagnosed in 6 adults by histology/immunohistochemistry: diffuse large B-cell lymphoma (2), small B-cell lymphoma (2), concomitant follicular lymphoma and histiocytic sarcoma (1), and extraosseous plasmacytoma (1). Flow cytometry identified abnormal populations in 5 of 6 cases, and detected clonal populations in 2 reactive follicular hyperplasia cases., Conclusion: Tonsillar hematolymphoid malignancy is uncommon, and flow cytometry was less accurate than histology/immunohistochemistry for its diagnosis. Despite the rarity of tonsillar lymphoma in children, nearly half of study patients were pediatric. Intraoperative frozen section diagnosis showed excellent sensitivity for malignancy, and could be used to effectively triage cases for flow cytometry evaluation.

Published

2017

6. Genesis of the Special Issues on Mass Cytometry.

Author

Preffer F and Tarnók A

Subjects

Flow Cytometry methods, Periodicals as Topic

Published

2017

7. A novel approach to measuring cell-mediated lympholysis using quantitative flow and imaging cytometry.

Author

La Muraglia GM 2nd, O'Neil MJ, Madariaga ML, Michel SG, Mordecai KS, Allan JS, Madsen JC, Hanekamp IM, and Preffer FI

Subjects

Animals, Cells, Cultured, Swine, Swine, Miniature, Cytotoxicity Tests, Immunologic methods, Cytotoxicity, Immunologic immunology, Flow Cytometry methods, Stem Cells immunology, T-Lymphocytes, Cytotoxic immunology

Abstract

In this study, we established a novel isotope-free approach for the detection of cell-mediated lympholysis (CML) in MHC defined peripheral blood mononuclear cells (PBMCs) using multiparameter flow and imaging cytometry. CML is an established in vitro assay to detect the presence of cytotoxic effector T-lymphocytes precursors (CTLp). Current methods employed in the identification of CTLp in the context of transplantation are based upon the quantification of chromium ((51)Cr) released from target cells. In order to adapt the assay to flow cytometry, primary porcine PBMC targets were labeled with eFluor670 and incubated with major histocompatibility complex (MHC) mismatched effector cytotoxic lymphocytes (CTLs). With this method, we were able to detect target-specific lysis that was comparable to that observed with the (51)Cr-based assay. In addition, the use of quantitative cell imaging demonstrates the presence of accessory cells involved in the cytotoxic pathway. This innovative technique improves upon the standard (51)Cr release assay by eliminating the need for radioisotopes and provides enhanced characterization of the interactions between effector and target cells. This technique has wide applicability to numerous experimental and clinical models involved with effector-cell interactions., (Copyright © 2015 Elsevier B.V. All rights reserved.)

Published

2015

8. The role of CD19 and CD27 in the diagnosis of multiple myeloma by flow cytometry: a new statistical model.

Author

Cannizzo E, Carulli G, Del Vecchio L, Ottaviano V, Bellio E, Zenari E, Azzarà A, Petrini M, and Preffer F

Subjects

Antineoplastic Combined Chemotherapy Protocols therapeutic use, Biomarkers, Tumor metabolism, Bone Marrow metabolism, Bone Marrow pathology, Bone Marrow Transplantation, Clone Cells, Combined Modality Therapy, Humans, Models, Statistical, Multiple Myeloma metabolism, Multiple Myeloma therapy, Prospective Studies, Treatment Outcome, Antigens, CD19 metabolism, Flow Cytometry methods, Multiple Myeloma diagnosis, Tumor Necrosis Factor Receptor Superfamily, Member 7 metabolism

Abstract

We have developed a new statistical diagnostic model that examines the correlation between immunophenotype and clonality as detected by flow cytometry (FC) and histology, defining the diagnostic role of FC in multiple myeloma (MM). The 192 bone marrow samples from patients and control subjects were studied for routine diagnostic analysis of MM; a minimum of 100 plasma cells (PCs) were analyzed for each patient sample. A direct 7- or 8-color method was applied to study the immunophenotype of PCs, utilizing a FACSCanto II (BD Biosciences, San Jose, CA). Samples were labeled with fluorochrome-conjugated monoclonal antibodies (AmCyan, Pac Blue, fluorescein isothiocyanate, phycoerythrin [PE], PECy7, peridinin-chlorophyll protein, allophycocyanin [APC], and APC-Cy7) to the following antigens: CD138, CD81, CD200, CD221, CD45, CD38, CD28, CD19, CD27, CD117, CD38, CD33, CD20, CD56, CD10, and immunoglobulin κ and λ light chains. Among all antigens tested, CD19 and CD27, when applied to our model, resulted in optimal concordance with histology. This model defines the effective diagnostic role FC could have in MM and in the detection of minimal residual disease.

Published

2012

9. Physics of a rapid CD4 lymphocyte count with colloidal gold.

Author

Hansen P, Barry D, Restell A, Sylvia D, Magnin O, Dombkowski D, and Preffer F

Subjects

Animals, Fluorescent Antibody Technique, Humans, Mice, Microscopy, Fluorescence methods, CD4 Lymphocyte Count methods, CD4-Positive T-Lymphocytes, Flow Cytometry methods, Gold Colloid

Abstract

The inherent surface charges and small diameters that confer colloidal stability to gold particle conjugates (immunogold) are detrimental to rapid cell surface labeling and distinct cluster definition in flow cytometric light scatter assays. Although the inherent immunogold surface charge prevents self aggregation when stored in liquid suspension, it also slows binding to cells to timeframes of hours and inhibits cell surface coverage. Although the small diameter of immunogold particles prevents settling when in liquid suspension, small particles have small light scattering cross sections and weak light scatter signals. We report a new, small particle lyophilized immunogold reagent that maintains activity after 42°C storage for a year and can be rapidly dissolved into stable liquid suspension for use in labelling cells with larger particle aggregates that have enhanced scattering cross section. Labeling requires less than 1 min at 20°C, which is ∼30 times faster than customary fluorescent antibody labeling. The labeling step involves neutralizing the surface charge of immunogold and creating specifically bound aggregates of gold on the cell surface. This process provides distinct side-scatter cluster separation with blue laser light at 488 nm, which is further improved by using red laser light at 640 nm. Similar comparisons using LED light sources showed less improvement with red light, thereby indicating that coherent light scatter is of significance in enhancing side-scatter cluster separation. The physical principles elucidated here for this technique are compatible with most flow cytometers; however, future studies of its clinical efficacy should be of primary interest in point-of-care applications where robust reagents and rapid results are important., (Copyright © 2011 International Society for Advancement of Cytometry.)

Published

2012

10. Multiparameter immunophenotyping by flow cytometry in multiple myeloma: The diagnostic utility of defining ranges of normal antigenic expression in comparison to histology.

Author

Cannizzo E, Bellio E, Sohani AR, Hasserjian RP, Ferry JA, Dorn ME, Sadowski C, Bucci JJ, Carulli G, and Preffer F

Subjects

Antibodies, Monoclonal immunology, Confidence Intervals, Humans, Multiple Myeloma pathology, Plasma Cells immunology, Plasma Cells pathology, Reference Values, Antigens, Neoplasm immunology, Flow Cytometry methods, Immunophenotyping methods, Multiple Myeloma diagnosis, Multiple Myeloma immunology

Abstract

Background: Numerous studies have reported on the immunophenotype of plasma cells (PCs) in monoclonal gammopathy of undetermined significance (MGUS) and in plasma cell myeloma (PCM), but very few have examined the immunophenotype of normal PCs. In this study, an objective definition of normal range of expression for each antigen was found on normal control PCs. Using these new ranges of normal expression (new method) is different from using a static 20% of PCs cut-off for all antigens as described in the literature (traditional method). These newly calculated normal ranges for each antigen were applied to our data, and compared to histologic and immunohistochemical findings., Methods: Bone marrow samples from 46 patients with PC neoplasms and 15 normal controls were studied. A minimum of 100 PC were analyzed for each patient and control sample. An 8-color staining method was applied to study the immunophenotype of PCs, using a BD FACSCanto II., Results: By the new ranges of normality calculated in this study it was determined that different antigens have different level of expression on polyclonal PCs. CD19 correlated with histology by both the traditional and new methods, but had superior correlation by the new method., Conclusions: This report is the first 8-color immunophenotypic study of PCM in which a "range of normal expression" for each antigen is defined. This is a critical step to help distinguish between a normal and neoplastic PC immunophenotype and discern which antigens are of diagnostic importance., ((c) 2010 Clinical Cytometry Society.)

Published

2010

11. When monocytes and platelets compete: The effect of platelet count on the flow cytometric measurement of monocyte CD36.

Author

Dzik WH, Cserti-Gazdewich CM, Ssewanyana I, Delelys M, and Preffer FI

Subjects

CD36 Antigens immunology, Humans, Monocytes cytology, Platelet Count, Sensitivity and Specificity, Blood Platelets cytology, Blood Platelets metabolism, CD36 Antigens blood, Flow Cytometry methods, Monocytes metabolism

Abstract

Background: Flow cytometric measurement of monocyte surface CD36 is relevant to several conditions including diabetes, cardiovascular disease, lipid disorders, platelet isoimmunization, and susceptibility to P falciparum malaria. CD36 is also strongly expressed on platelets where it is also known as platelet glycoprotein IV., Methods: Whole blood samples, containing identical monocyte concentrations, were adjusted to contain platelets ranging from 20,000/uL to 600,000/uL, were stained with fluorescent-labeled anti-CD36, and analyzed by flow cytometry., Results: CD36 median fluorescent intensity (MFI) observed on monocytes decreased as the platelet concentration in the sample increased with more than a 50% decline in monocyte MFI over the normal range of platelet values. The effect was not abolished by using larger volumes of monoclonal antibody and was observed with different clones of reagent anti-CD36. The findings were most consistent with competition by platelets for the CD36 reagent. Similar findings were observed with antibody to class I HLA. Under defined assay conditions, monocyte CD36 MFI declined with rising platelet concentration in a predictable fashion following an inverse linear relationship., Conclusions: Measurement of CD36 expression on monocytes by flow cytometry in whole blood samples is affected by the sample platelet count. When comparing the monocyte CD36 expression among different individuals, our approach can be used to adjust measured monocyte CD36 expression for the effect of the platelet concentration in the sample. Competition by platelets for monoclonal reagents may occur in other settings when whole blood assays are used and when the target antigen is strongly expressed on both platelets and leukocytes., ((c) 2009 Clinical Cytometry Society.)

Published

2010

12. Flow cytometry and the stability of phycoerythrin-tandem dye conjugates.

Author

Hulspas R, Dombkowski D, Preffer F, Douglas D, Kildew-Shah B, and Gilbert J

Subjects

Biotin chemistry, CD4-Positive T-Lymphocytes cytology, CD8-Positive T-Lymphocytes cytology, Cell Separation, Fluorescence Resonance Energy Transfer, Fluorescent Dyes chemistry, Humans, Leukocytes, Mononuclear cytology, Polystyrenes chemistry, T-Lymphocytes, Regulatory cytology, Coloring Agents pharmacology, Flow Cytometry methods, Phycoerythrin chemistry, T-Lymphocytes cytology

Abstract

Routine clinical flow cytometric procedures demand rigorous, simple, and reproducible procedures for spectral compensation. The current, often laborious, spectral compensation procedures are the result of variability in instrument settings, instrument performance, and variability in reagents. In particular, the use of tandem dye conjugates necessitates elaborate spectral compensation procedures that need to be applied frequently. Manufacturer, lot number, and handling procedures are considered the key aspects affecting the fluorescence characteristics of tandem dyes. A better understanding of how specific conditions affect the variability in emission spectra of tandem dyes can lead to a considerable increase in reliability of measurements and a potential simplification of setup procedures for routine, clinical flow cytometry. We investigated the effect of light exposure, handling, and storage conditions on the fluorescence characteristics of some common phycoerythrin tandem fluorochromes. In general, PE-Cy5 showed the lowest degradation rates, whereas PE-Cy7 showed the highest. During storage, long-term degradation rates were lowest for reagents packaged using an extra light protective approach. Under these conditions, a degradation rate of 0.9%/month of a PE-Cy7 conjugate decreased to 0.3%/month. As degradation rates were minimized, we studied the effect of slow degradation of a set of tandem dye conjugates on compensation matrix values over several months. Finally, we explored the effect of slow degradation on flow cytometric analysis using the same compensation settings for extended periods for an analysis template with preset regions and gating strategies., (Copyright 2009 International Society for Advancement of Cytometry.)

Published

2009

13. Advances in complex multiparameter flow cytometry technology: Applications in stem cell research.

Author

Preffer F and Dombkowski D

Subjects

Animals, Biomedical Research methods, Flow Cytometry methods, Humans, Mice, Microscopy, Fluorescence, Rats, Software, Biomedical Research instrumentation, Flow Cytometry instrumentation, Stem Cells cytology, Stem Cells physiology

Abstract

Flow cytometry and cell sorting are critical tools in stem cell research. Recent advances in flow cytometric hardware, reagents, and software have synergized to permit the stem cell biologist to more fully identify and isolate rare cells based on their immunofluorescent and light scatter characteristics. Some of these improvements include physically smaller air-cooled lasers, new designs in optics, new fluorescent conjugate-excitation pairs, and improved software to visualize data, all which combine to open up new horizons in the study of stem cells, by enhancing the resolution and specificity of inquiry. In this review, these recent improvements in technology will be outlined and important cell surface and functional antigenic markers useful for the study of stem cells described., ((c) 2009 Clinical Cytometry Society.)

Published

2009

14. Fine-needle aspiration biopsy in the diagnosis and classification of primary and recurrent lymphoma: a retrospective analysis of the utility of cytomorphology and flow cytometry.

Author

Dong HY, Harris NL, Preffer FI, and Pitman MB

Subjects

Biopsy, Needle, False Negative Reactions, False Positive Reactions, Humans, Lymph Nodes pathology, Reproducibility of Results, Retrospective Studies, Flow Cytometry, Image Cytometry, Lymphoma classification, Lymphoma diagnosis

Abstract

We retrospectively reviewed our experience with the fine-needle aspiration biopsy (FNAB) diagnosis of primary and recurrent lymphoma to assess the ability of cytomorphology with and without ancillary flow cytometry (FCM) analysis to diagnose and subclassify these tumors according to the Revised European-American Lymphoma/World Health Organization classifications. We reviewed 139 consecutive FNABS of 84 primary and 55 recurrent lymphomas. FCM was successful in 105 (75%) cases. The overall results, including cases without FCM, included 93/139 (67%) true positive, 7 (5%) false negative, and 39 indeterminate (27 [19%] suspicious and 12 [9%] atypical) diagnoses of lymphoma. In cases with FCM, there were 80/105 (77%) true positive, no false negative, and 25 indeterminate diagnoses (15 [14%] suspicious and 10 [9%] atypical). The overall results of the 84 primary lymphomas were 55 (67%) true positive, 5 (5%) false negative, and 24 indeterminate (14[16%] suspicious and 10 [12%] atypical) diagnoses for lymphoma. Of the 68 primary lymphomas analyzed with FCM, 50 [74%] were true positives, and 28 were indeterminate (11 [16%] suspicious and 7 [10%] atypical). There were no false negatives. Diagnostic accuracy varied among lymphoma subtypes. Subclassification of the positive cases were initially conclusive in only 55/93 cases (59%). However, a retrospective review of the morphologic together with FCM data in 15 of the 23 unclassified cases improved the overall subclassification of positive cases to 77%. Subclassification was best in small lymphocytic lymphoma/chronic lymphocytic leukemia, lymphoplasmacytic lymphoma, Burkitt's lymphoma, mantle cell lymphoma, and plasmacytoma (all 100%). Subclassification was poor in marginal-zone lymphoma (33%), and initially as well in diffuse large B-cell lymphoma (62%), but it improved on review (95%), as did subclassification of follicular lymphoma (77 to 100% on review). Hodgkin's disease was recognized as malignant in only 44% of the cases (7/16) and was classified as such based on morphology alone. This review of our early efforts to diagnose and subclassify lymphoma with FNAB and FCM indicates that although a diagnosis and proper subclassification of lymphoma can be made with certainty in the majority of cases, recurrent or primary, it requires close coordination of cytomorphology and immunophenotyping data, which often comes with close cooperation of cytopathologists and hematopathologists. A mere cytological diagnosis of positive for lymphoma is no longer acceptable if FNAB is to become an independent diagnostic tool for lymphoma.

Published

2001

15. Flow cytometric DNA ploidy and cells phase fractions in recurrent human pituitary adenomas. A correlative study of flow cytometric analysis and the expression of proliferating cell nuclear antigen.

Author

Chae YS, Flotte T, Hsu DW, Preffer F, and Hedley-Whyte ET

Subjects

Adenoma pathology, Adult, Aged, Female, Genetic Markers genetics, Humans, Immunohistochemistry, Male, Middle Aged, Pituitary Neoplasms pathology, Proliferating Cell Nuclear Antigen analysis, Adenoma genetics, Biomarkers, Tumor analysis, Cell Cycle genetics, DNA, Neoplasm analysis, Flow Cytometry methods, Mitotic Index genetics, Neoplasm Recurrence, Local genetics, Pituitary Neoplasms genetics, Ploidies

Abstract

Flow cytometric analysis was applied to embedded tissue to measure the proliferative activity and the DNA ploidy of 16 recurrent and 17 nonrecurrent pituitary adenomas. The results were compared with data from a previous study which demonstrated that proliferating cell nuclear antigen (PCNA) labeling index was higher in recurrent adenomas than in nonrecurrent adenomas. Flow cytometric analysis as a tool for predicting aggressive behavior has been useful in a variety of human tumors; however, its prognostic value in pituitary adenomas is controversial. Therefore, we decided to explore the relationship of the results of flow cytometry and proliferating cell nuclear antigen labeling indices with the prognosis of pituitary adenomas. Three out of 16 recurrent adenomas and five out of 17 nonrecurrent adenomas demonstrated a DNA aneuploid pattern. All the nonfunctional recurrent adenomas had a diploid pattern, while only 40% of the functional recurrent adenomas had a diploid pattern. The GO/G1 phase fraction was higher in the recurrent adenomas, than in the nonrecurrent ones (p = 0.0005). In contrast, the S-phase fraction and the coefficient of variation were higher in the nonrecurrent adenomas (5.9 +/- 1.0%, 7.0 +/- 0.75, respectively) than in the recurrent ones (2.5 +/- 0.6%, 4.0 +/- 0.2%, respectively) (p = 0.003 and p = 0.001, respectively). The proliferating cell nuclear antigen labeling indices were higher in the recurrent adenomas (18.9 +/- 4.5%) than in the nonrecurrent adenomas (2.6 +/- 1.6%) (p = 0.003). The S-phase of flow cytometry correlated weakly with the proliferating cell nuclear antigen labeling indices when the recurrent and the nonrecurrent adenomas were considered as one group. (r = -0.356, p = 0.033). But no significant correlations were observed when the groups of recurrent (r = -0.311, p = 0.195) and nonrecurrent tumors (r = -0.019, p = 0.942) were compared separately. The results of flow cytometric analysis suggest that recurrent adenomas may have a higher proportion of cells in the presynthetic phase than the nonrecurrent adenomas. This study suggests that flow cytometric analysis is of limited value in predicting recurrence of pituitary adenomas.

Published

1996

16. DNA flow cytometry of primary tumors and their skin metastases. Correlation of DNA histograms.

Author

Flotte TJ, Pastel-Levy C, Graeme-Cook F, Preffer F, and Bell DA

Subjects

Aneuploidy, Carcinoma pathology, Cell Nucleus chemistry, Diploidy, G1 Phase, Humans, Neoplasms, Multiple Primary genetics, Neoplasms, Multiple Primary pathology, Resting Phase, Cell Cycle, Skin Neoplasms pathology, Carcinoma genetics, Carcinoma secondary, DNA, Neoplasm analysis, Flow Cytometry, Skin Neoplasms genetics, Skin Neoplasms secondary

Abstract

The purpose of this study was to determine whether quantification of DNA content would demonstrate conserved patterns in primary tumors and their metastases and to learn whether this technique would be useful in determining if a tumor was metastatic from a previous primary tumor or represented a new neoplasm. The study comprised of all cases nonmelanoma metastatic skin lesions in which the primary tumor was also resected at this hospital between the years 1984 and 1990 (22 cases). Both the primary and metastatic lesions were examined by the deparaffinized flow cytometric technique for DNA content. DNA-aneuploid tumors were considered to correlate if the DNA indices (ratio of aneuploid to diploid peak channels) were within 10%. Thirty-four tumors were DNA-aneuploid; eight tumors were DNA-diploid. We found agreement in 20 of 22 cases (agree--aneuploid: 16 cases; agree--diploid: four cases). In six of our cases the histograms of the primary and the metastatic lesions did not correlate when only one block was examined; however, when three blocks from each site were studied, we found concordance of DNA indices in four cases. There was disagreement in two of 22 cases (disagree--different DNA indices: two cases). In both of these cases, only one block of the primary tumor was available for examination, and the histograms were of marginal quality. This study demonstrates that the histogram pattern (aneuploid versus diploid) of DNA content is highly conserved between primary and metastatic tumors. There was 91% agreement between DNA indices of primary tumors and their metastases (20 of 22 cases) using a 10% correlation criterion.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1992

17. Application of DNA flow cytometry from paraffin-embedded tissue to the diagnosis of mycosis fungoides.

Author

Pastel-Levy C, Flotte TJ, Preffer F, Ware A, Graeme-Cook F, Bell DA, and Colvin RB

Subjects

Aneuploidy, Cell Division, DNA, Neoplasm analysis, Histological Techniques, Humans, Mycosis Fungoides chemistry, Mycosis Fungoides genetics, Paraffin, Prognosis, Skin Neoplasms chemistry, Skin Neoplasms genetics, DNA, Neoplasm genetics, Flow Cytometry, Mycosis Fungoides diagnosis, Skin Neoplasms diagnosis

Abstract

The distinction of mycosis fungoides from benign inflammatory lesions is sometimes difficult by conventional histological techniques. Aneuploidy, a feature often associated with malignant tumors, can be assessed even in tissue routinely processed in paraffin using the flow cytometric technique of Hedley and associates. In many tumor systems, there are significant diploid clones. We have evaluated the flow cytometric DNA ploidy of paraffin-embedded tissue in the diagnosis and prognosis of mycosis fungoides (MF). We studied 22 cases of MF and 10 control cases of inflammatory skin lesions with epidermal involvement. Aneuploidy was found in 27% of the MF cases, but in none of the controls (ED). Aneuploid features were seen in 23% of tissues from early stage disease. Aneuploidy did not correlate with atypia, epidermotropism, or number of mitoses. There was a trend towards showing adverse outcome in those patients with aneuploid lesions. The detection of aneuploidy might be helpful for early diagnosis of MF.

Published

1991

18. New technologies in cell analysis by flow cytometry.

Author

Colvin RB and Preffer FI

Subjects

Antibodies, Monoclonal, Antigens, Surface analysis, Biopsy, Needle, Chromosomes analysis, DNA metabolism, Flow Cytometry instrumentation, Fluorescent Dyes, Humans, Flow Cytometry methods

Abstract

Automated flow cytometry provides an efficient, sensitive, objective, and quantitative means to analyze cells and their components in suspension. Two major diagnostic applications are the identification of cells in the blood by monoclonal antibodies to surface molecules and the characterization of tumor cell ploidy by nuclear DNA analysis. New technologies permit analysis of small quantities of cells (as in fine-needle aspirates), multiple simultaneous markers, oncogene products, and paraffin-embedded tissue. The technique has become the standard for cells normally in suspension (blood, other fluids). For cells readily obtained in suspension (fine-needle aspirates, nuclei), flow cytometry offers a practical alternative to computer-assisted microscopy.

Published

1987

19. Is it time to revisit our current hematopoietic progenitor cell quantification methods in the clinic?

Author

Beksac, M and Preffer, F

Published

2012

20. Occurrence of melanoma in "dysplastic" nevus spilus: report of case and analysis by flow cytometry.

Author

Kurban, R. S., Preffer, F. I., Sober, A. J., Mihm Jr., M. C., and Barnhill, R. L.

Subjects

*MELANOMA, *NEUROENDOCRINE tumors, *DYSPLASIA, *FLOW cytometry, *CYTOLOGICAL techniques, *PLOIDY

Abstract

We report a case of melanoma arising in a large nevus spilus. On histologic examination, the nevus spilus had diagnostic features of melanocylic dysplasia. Further characterization by flow cytometry showed DNA-aneuploidy within the melanoma as well as in one of the darker pigmented papules within the nevus spilus. The significance of this finding and a review of melanomas originating in nevi spili are presented. [ABSTRACT FROM AUTHOR]

Published

1992

21. The role of CD19 and CD27 in the diagnosis of Multiple Myeloma by Flow Cytometry: a new statistical model

Author

Virginia Ottaviano, Mario Petrini, Elisa Cannizzo, Giovanni Carulli, Frederic I. Preffer, Emanuele Bellio, Luigi Del Vecchio, Antonio Azzara, Ezio Zenari, Cannizzo, E., Carulli, G., DEL VECCHIO, Luigi, Ottaviano, V, Bellio, E, Zenari, E, Azzarà, A, Petrini, M, and Preffer, F.

Subjects

Pathology, medicine.medical_specialty, medicine.drug_class, Antigens, CD19, Monoclonal antibody, Flow cytometry, chemistry.chemical_compound, Immunophenotyping, immune system diseases, Bone Marrow, hemic and lymphatic diseases, Antineoplastic Combined Chemotherapy Protocols, medicine, Biomarkers, Tumor, Humans, Prospective Studies, Fluorescein isothiocyanate, Multiple myeloma, Bone Marrow Transplantation, Allophycocyanin, Models, Statistical, medicine.diagnostic_test, biology, General Medicine, medicine.disease, Flow Cytometry, Minimal residual disease, Molecular biology, Combined Modality Therapy, Clone Cells, Tumor Necrosis Factor Receptor Superfamily, Member 7, Treatment Outcome, chemistry, biology.protein, Antibody, Multiple Myeloma

Abstract

We have developed a new statistical diagnostic model that examines the correlation between immunophenotype and clonality as detected by flow cytometry (FC) and histology, defining the diagnostic role of FC in multiple myeloma (MM). The 192 bone marrow samples from patients and control subjects were studied for routine diagnostic analysis of MM; a minimum of 100 plasma cells (PCs) were analyzed for each patient sample. A direct 7- or 8-color method was applied to study the immunophenotype of PCs, utilizing a FACSCanto II (BD Biosciences, San Jose, CA). Samples were labeled with fluorochrome-conjugated monoclonal antibodies (AmCyan, Pac Blue, fluorescein isothiocyanate, phycoerythrin [PE], PECy7, peridinin-chlorophyll protein, allophycocyanin [APC], and APC-Cy7) to the following antigens: CD138, CD81, CD200, CD221, CD45, CD38, CD28, CD19, CD27, CD117, CD38, CD33, CD20, CD56, CD10, and immunoglobulin κ and λ light chains. Among all antigens tested, CD19 and CD27, when applied to our model, resulted in optimal concordance with histology. This model defines the effective diagnostic role FC could have in MM and in the detection of minimal residual disease.

Published

2011