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3. Fluorescent in vivo tracking of hematopoietic cells. Part I. Technical considerations

Author

Slezak, SE and Horan, PK

Abstract

We report a new technology for in vivo tracking of hematopoietic cells, using fluorescent lipophilic probes. Because the probe is irreversibly bound in the lipids of the cell membrane; substantial numbers of dye molecules can be incorporated per cell and thus substantial signal to noise can be achieved. Although this technology can be used for all hematopoietic cells, these first findings are reported on red blood cells (RBCs) owing to the importance of the membrane to RBC function and integrity. We demonstrated that labeling 10% of the RBCs of a rabbit and reinjecting them into the animal makes possible the tracking of these cells at various times after injection. Furthermore, the labeling appears not to affect in vivo cell lifetime or cellular volume changes in response to hypotonic shock. The single cell fluorescence intensity of the labeled RBCs remains relatively constant for 60 days, and an immune response appears not to be generated against labeled cells. That labeled RBCs have lifetime kinetics in vivo, as shown in other studies, indicates that the membranes are functioning normally and are unaltered by the labeling technology. The technology we present is also applicable to white blood cells, bone marrow, and platelets.

Published
1989
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4. Mechanisms of adoptive immunotherapy: improved methods for in vivo tracking of tumor-infiltrating lymphocytes and lymphokine-activated killer cells.

Author

Wallace PK, Palmer LD, Perry-Lalley D, Bolton ES, Alexander RB, Horan PK, Yang JC, and Muirhead KA

Subjects
Animals, Cell Division drug effects, Cell Division physiology, Female, Flow Cytometry, Fluorescent Dyes pharmacokinetics, Fluorescent Dyes pharmacology, Iodine Radioisotopes, Killer Cells, Lymphokine-Activated drug effects, Killer Cells, Lymphokine-Activated physiology, Lung metabolism, Lung Neoplasms metabolism, Lung Neoplasms secondary, Lung Neoplasms therapy, Lymphocytes, Tumor-Infiltrating drug effects, Lymphocytes, Tumor-Infiltrating physiology, Mice, Mice, Inbred C57BL, Models, Biological, Neoplasms, Experimental metabolism, Neoplasms, Experimental therapy, Tissue Distribution, Immunotherapy, Adoptive methods, Killer Cells, Lymphokine-Activated metabolism, Lymphocytes, Tumor-Infiltrating metabolism, Organic Chemicals
Abstract

Adoptive immunotherapy with tumor-infiltrating lymphocytes (TIL) and lymphokine-activated killer cells has been demonstrated to mediate regression of tumors in murine models and in selected patients with advanced cancer. Improved methods for monitoring immune cell traffic, particularly to sites of tumor, are needed to elucidate mechanisms of antitumor activity and optimize treatment protocols. Traditional cell tracking methods such as fluorescent protein labeling and radiolabeling using 111In, 125I, or 51Cr are limited by isotope half-life, leakage or transfer of label from immune cells, and toxicity or altered cell function caused by the labeling process. Labeling with genetic markers allows long-term cell tracking but is laborious to perform and difficult to quantitate. We have used two recently described lipophilic cell tracking compounds (PKH26 and 125I-PKH95) which stably partition into lipid regions of the cell membrane to track immune cells in vivo. Concentrations of each tracking compound which had no adverse effects were determined for a variety of murine TIL and lymphokine-activated killer cell functions. Viability was unimpaired at labeling concentrations of up to 5 microM for PKH95 and 20 microM for PKH26. TIL proliferation was unaltered by labeling with up to 5 microM PKH95, 20 microM PKH26, or a combination of 15 microM PKH26 and 5 microM PKH95. In vivo cytotoxic effector function and in vivo therapeutic efficacy of lymphokine-activated killer cells and TIL were also unimpaired by labeling with 20 microM PKH26 or 1 microM 125I-PKH95. Subsequent studies in an adoptive transfer immunotherapy model used 125I-PKH95 to track the biodistribution of TIL in tumor and in non-tumor-bearing animals and PKH26 fluorescence to monitor microdistribution within tissues and distinguish TIL from host T-cells. The results suggest that differential accumulation, selective retention, or proliferation at the tumor site cannot account for the observed pattern of therapeutic efficacy. We hypothesize that a minimum number of TIL must reach the tumor site in order to achieve a demonstrable therapeutic effect.

Published
1993

5. Cell cycle analysis of asexual stages of erythrocytic malaria parasites.

Author

Jacobberger JW, Horan PK, and Hare JD

Subjects
Animals, DNA, Protozoan analysis, Female, Flow Cytometry, G1 Phase, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, S Phase, Cell Cycle, Erythrocytes parasitology, Malaria blood, Malaria parasitology, Plasmodium chabaudi cytology, Plasmodium chabaudi growth & development
Abstract

Intra-erythrocytic Plasmodium species can be stained with the DNA binding dye, Hoechst 33342, and the distribution of DNA content determined for parasite populations by flow cytometric measurement of fluorescence. Analysis of this distribution will determine the parasitaemia (percentage of erythrocytes infected), and the percentages of trophozoite infected red blood cells, polyparasitized (trophozoite) red blood cells, and schizont/segmenter infected red blood cells. This analysis is based on the hypothesis that the asexual parasites cycle with single G1 period, and effectively, a single S phase with no significant G2/M period except at schizogony when the genome DNA content is equivalent to 8 N or higher, dependent on the species. Data are presented to support this model.

Published
1992
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6. Long-term tracking of lymphocytes in vivo: the migration of PKH-labeled lymphocytes.

Author

Teare GF, Horan PK, Slezak SE, Smith C, and Hay JB

Subjects
Animals, Cell Movement, Cell Survival, Flow Cytometry, Lymph cytology, Microscopy, Fluorescence, Organic Chemicals, Sheep, Time Factors, Fluorescent Dyes, Lymphocytes physiology
Abstract

Studies of in vivo cell migration using cell markers such as 51Cr, 111In, FITC, or XRITC have been limited to short time periods due to the elution, toxicity, or rapid loss of label detectability. We have labeled sheep lymphocytes in vitro with PKH-2, a new fluorescent cell membrane label, and, after their intravenous injection back into donor sheep, have been able to detect them in efferent lymph, using flow cytometry, for longer than 38 days. The PKH-2-labeled lymphocytes migrated with similar kinetics, efficiency, and tissue specificity as lymphocytes labeled with cell markers used previously. PKH-2-labeled cells mediated graft versus host reactions indistinguishable from those mediated by unlabeled cells, and cell surface antigens were equally detectable on the surface of labeled and unlabeled lymphocytes. According to the slow, consistent loss of fluorescence intensity of the labeled cells in vivo, we predict that labeled lymphocytes could remain detectable by flow cytometry for greater than 7 weeks with the labeling protocol used in these experiments.

Published
1991
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7. Fluorescent cell labeling for in vivo and in vitro cell tracking.

Author

Horan PK, Melnicoff MJ, Jensen BD, and Slezak SE

Subjects
Animals, Blood Platelets, Cells, Cultured, Endocytosis, Mice, Organic Chemicals, Phagocytes, Rabbits, Reagent Kits, Diagnostic, Specimen Handling, Cell Movement, Flow Cytometry methods, Fluorescent Dyes pharmacokinetics, Membrane Lipids
Published
1990
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8. Analysis of malaria parasite-infected blood by flow cytometry.

Author

Jacobberger JW, Horan PK, and Hare JD

Subjects
Animals, Benzimidazoles, Cell Fractionation, Female, Mice, Mice, Inbred Strains, Staining and Labeling, Erythrocytes parasitology, Flow Cytometry, Malaria parasitology
Abstract

The use of flow cytometry in the quantitative analysis of blood from mice infected with Plasmodium vinckei has been studied. Several fluorescent dyes responsive to cell membrane potential were screened and one dye, 3,3'-dimethyloxacarbocyanine (DiOC1(3) ), was chosen for further study. Mature red blood cells (mRBC), immature RBC (imRBC), and parasitized RBC (pRBC) could be recognized and counted in the flow cytometer. When infected blood was separated on a Percoll gradient and fractions analyzed by flow cytometry using DiOC1(3), distinct populations of pRBC were recognized, the frequency of which varied with density. These subpopulations could not be correlated with distinct morphologic stages but varied with the size or age of the growing parasite. Methods combining the use of DiOC1(3) with a DNA specific-dye, Hoechst 33342, are discussed as an approach to more complete analysis of the blood of malaria-infected animals.

Published
1983
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9. Cell-mediated cytotoxicity. A highly sensitive and informative flow cytometric assay.

Author

Slezak SE and Horan PK

Subjects
Animals, Chromium Radioisotopes, Female, Fluorescence, Killer Cells, Natural immunology, Mice, Mice, Inbred C3H, Cytotoxicity, Immunologic, Flow Cytometry
Abstract

Determination of target cell lysis by cytolytic effectors has typically been achieved by two methods: the release of various markers from the cell, as in 51chromium release assays and the uptake of markers into the cell, as in trypan blue uptake in single cell/conjugate binding assays. Problems associated with these assays might include: (1) poor uptake, (2) nonspecific release, (3) poor statistics, (4) length of assays, or (5) subjectivity. These difficulties prompted the development of a new sensitive flow cytometric assay employing two fluorochromes. PKH-1, a fluorochrome which fluoresces in the green, binds to the cytoplasmic membrane and does not leak or transfer, is used to identify the target cell population. Propidium iodide fluoresces in the red and is used to detect non-viable cells. Use of these two fluorochromes and two parameter analysis allows for identification of four subpopulations in the sample: live effectors, dead effectors, live targets and dead targets. By enumeration of these subpopulations the following information can be calculated: (1) the percent target lysis, (2) effector-to-target cell ratios, (3) viability of the effector cells at the termination of the assay, and (4) viable effector to target cell ratios. The results show that PKH-1 labeling of target cells had no effect on effector-target cell interactions. Excellent correlation was found between this method and the chromium assay, however, due to earlier detection of the lytic event, this method provides a distinct time advantage over current methods.

Published
1989
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10. Maintenance of peritoneal macrophages in the steady state.

Author

Melnicoff MJ, Horan PK, Breslin EW, and Morahan PS

Subjects
Animals, Antibodies, Monoclonal, Cell Count, Cell Division, Female, Fluorescent Antibody Technique, Mice, Mice, Inbred BALB C, Neutrophils cytology, Peritoneal Cavity cytology, Staining and Labeling, Macrophages cytology
Abstract

Resident peritoneal macrophages (M phi) were labeled in situ by intraperitoneal (i.p.) injection of the green fluorescent cell tracking dye PKH-1. After immunofluorescence staining with M phi specific monoclonal antibodies (Mabs) and phycoerythrin (PE) second antibody, the resident M phi were labeled with both the green dye and red Mab label, while recruited M phi were labeled only with the red Mab tag. These populations were distinguished by two-color flow cytometry. PKH-1 labeled resident peritoneal M phi were followed for 1-49 days in mice that received no further treatment (steady state). Dye labeled M phi were still detectable after 49 days in vivo, although their green fluorescence intensity had decreased steadily over time. The decrease in dye intensity was limited to M phi, as the fluorescence intensity of PKH-1 labeled peritoneal lymphocytes did not change. Resident M phi populations were clearly separated from recruited M phi by the intensity of their staining with PKH-1 for up to 28 days. No decrease in the number of resident (dye labeled) peritoneal M phi was observed over 1-28 days. These data indicate that resident peritoneal M phi were not replaced by recruited blood monocytes in the steady state.

Published
1988
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11. Antibody-bearing liposomes as multicolor immunofluorescence markers for flow cytometry and imaging.

Author

Truneh A, Machy P, and Horan PK

Subjects
Animals, Cell Line, Color, Fluorescein-5-isothiocyanate, Fluoresceins, H-2 Antigens analysis, HLA Antigens analysis, Histological Techniques, Humans, Mice, Microscopy, Fluorescence, Rhodamines, Thiocyanates, Antibodies, Monoclonal, Flow Cytometry, Fluorescent Antibody Technique, Liposomes administration & dosage
Abstract

Liposomes covalently coupled to monoclonal antibodies retain the specificity of the antibody and bind only to cells bearing the appropriate determinant. As opposed to directly labeled antibodies which generally have fluorochrome to protein ratio of between 2-5, the entrapped space inside liposome can contain several hundred to several thousand molecules of fluorochromes in a space chemically isolated from the outside environment, thus providing the potential for an amplified fluorescence signal. We have prepared small unilamellar liposomes containing the soluble fluorochromes carboxyfluorescein (CF), which fluoresces in the green and sulforhodamine (SR), which fluoresces in the red, and covalently coupled a series of monoclonal antibodies using a heterobifunctional reagent. We were able to detect, on an Epics 753 flow cytometer equipped with an argon ion and a dye laser and by fluorescence microscopy, both single and double labeled mouse spleen lymphocyte subsets, fibroblast L cells and Raji cells. Complete color separation was obtained with CF-labeled cells being detected only by the green photomultiplier and SR-labeled cells by the red photomultiplier. Cells labeled with both were detected by both photomultipliers. Liposomes bearing anti-Ia antibodies bound only to B lymphocytes whereas those with anti-H-2K antibody bound both to T and B lymphocytes. In another system, single and dual color immunofluorescence made possible the simultaneous detection of HLA and H-2K molecules on transfected murine fibroblast L cells. The signal-to-noise ratio was more favorable for the liposome-labeled reagents than reagents labeled with fluorescein isothiocyanate. Cells labeled with antibody-bearing liposomes could be fixed with paraformaldehyde or glutaraldehyde without adversely affecting the original staining patterns. Apart from the two fluorochromes described above, other markers of choice could be encapsulated without any adverse effect on the antibody-liposome coupling procedure or on the specificity of the conjugated antibody. Since the fluorochrome is not directly coupled to the protein, there is no requirement for protein conjugation sites in order for it be usefully encapsulated inside liposomes. Therefore, this system provides new opportunities to exploit different, as yet untapped fluorochromes for use in flow cytometry and imaging.

Published
1987
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12. Antitumor immunity induced by hybrid murine tumor cells: requirements for optimal immunization.

Author

McCune CS, O'Donnell RW, Horan PK, Budd HS, Spennacchio JL, Chuang C, and Henshaw EC

Subjects
Adenocarcinoma immunology, Adjuvants, Immunologic administration & dosage, Animals, Bacterial Vaccines administration & dosage, Cell Line, Female, Flow Cytometry, H-2 Antigens analysis, Kidney Neoplasms immunology, Kidney Neoplasms pathology, Mammary Neoplasms, Experimental pathology, Mice, Mice, Inbred C3H, Neoplasms, Experimental immunology, Propionibacterium acnes immunology, Hybrid Cells radiation effects, Immunization, Mammary Neoplasms, Experimental immunology
Abstract

Hybrid tumor cells have been evaluated for their ability to induce specific antitumor immunity in inbred female C3H/He mice challenged with the syngeneic BA tumor. Hybrid cells were produced by fusion of BA cells with a BALB/c renal adenocarcinoma, which is hypoxanthine phosphoribosyl transferase-deficient and grows well in culture. Corynebacterium parvum was evaluated as an adjuvant for BA and hybrid cells. The BA tumor was shown to be poorly immunogenic, and four weekly injections of BA cells alone or C. parvum alone did not confer significant immunity. When BA cells and C. parvum were mixed, survival time was prolonged and most mice remained tumor-free. Hybrid cell lines derived from the BA tumor were produced in culture in unlimited quantities and were successfully used as immunogens. The addition of C. parvum to hybrids gave a significant incremental increase in survival when compared to the survival resulting from immunization by hybrids without adjuvant. When hybrids without adjuvant were used, several weekly injections were required for effective immunization. Irradiated and unirradiated hybrids were compared, and it was found that irradiation did not diminish hybrid immunogenicity. The potential problems and advantages of this concept of therapy are discussed.

Published
1982

13. Long-term follow-up of donors cytapheresed more than 50 times.

Author

Heal JM, Horan PK, Schmitt TC, Bailey G, and Nusbacher J

Subjects
Adult, Aged, Aspartate Aminotransferases blood, Female, Ferritins blood, Follow-Up Studies, Humans, Iron blood, Leukocyte Count, Long-Term Care, Lymphocytes, Male, Middle Aged, Time Factors, Blood Donors, Cell Separation, Leukapheresis, Plateletpheresis
Abstract

11 volunteers who had donated white blood cells or platelets more than 50 times over a 5- to 9-year period were studied to determine whether any adverse consequences of many cytaphereses could be detected. Among the donors no significant differences were found in 18 hematological and biochemical parameters when compared to a group of age- and sex-matched nondonor controls. Despite extensive cumulative lymphocyte losses sustained by these donors, the ratio of T, B, helper and suppressor cells has been maintained within the normal range. No detrimental effects of multiple cytapheresis on the donors' health has been demonstrated to date.

Published
1983
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14. Evaluation of the S phase distribution of flow cytometric DNA histograms by autoradiography and computer algorithms.

Author

Sheck LE, Muirhead KA, and Horan PK

Subjects
Animals, Autoradiography, Cell Line, Cell Separation, Computers, Evaluation Studies as Topic, Lymphoma, Mice, Thymidine metabolism, DNA analysis, Flow Cytometry, Interphase
Abstract

Cell sorting and tritiated thymidine autoradiography were used to define the distribution of S phase cells in flow cytometric DNA histograms obtained from exponential mouse lymphoma cells (L5178Y). The numbers of labeled S phase cells, autoradiographically determined from cells sorted at 2-channel intervals in the G1/early S and late S/G2M regions of the histogram, were compared with the numbers of computed S phase cells in comparable 2-channel intervals as predicted by several computer algorithms used to extract cell cycle phase distributions from DNA histograms. Polynomial and multirectangle algorithms gave computed estimates of total %S in close agreement with the tritiated thymidine labeling index for the cell population, while multi-Gaussian algorithms underestimated %S. Interval autoradiographic and algorithm studies confirmed these results in that no significant differences were found between the autoradiographic S phase distribution and S phase distributions calculated by the polynomial and multirectangle models. However, S phase cells were significantly underestimated in G1/early S by a constrained multi-Gaussian model and in both G1/early S and late S/G2 by an unconstrained multi-Gaussian model. For the particular cell line (L5178Y), staining protocol (mithramycin following ethanol fixation) and instrumentation (Coulter TPS-2 cell sorter) used in this study, close agreement between computed %S and tritiated thymidine labeling index was found to be a reliable indicator of an algorithm's success in resolving S phase cells in the G1/S and S/G2 transition regions of the DNA histograms.

Published
1980
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15. A flow cytometric analysis of the embryonic origin of lymphocytes in diploid/triploid chimeric Xenopus laevis.

Author

Flajnik MF, Horan PK, and Cohen N

Subjects
Animals, Embryo, Nonmammalian physiology, Female, Flow Cytometry methods, Chimera, Diploidy, Lymphocytes physiology, Ploidies, Xenopus genetics
Abstract

Quantitative flow cytometry was used to examine the embryonic origin of lymphocytes in Xenopus laevis. Reciprocal head/body transplants were made between diploid (2N) and triploid (3N) embryos of the same developmental stages ranging from neural plate to tail bud stages. Thymuses and spleens were removed from postmetamorphic chimeras. Cell suspensions were stained with the fluorescent DNA stain, mithramycin, and the ploidy (relative fluorescence intensity) of the cells was then determined by flow cytometry. All lymphocytes in the chimeras were derived from the posterior portion of the embryo. In other experiments, various regions of the lateral plate or ventral mesoderm were grafted from triploid to diploid embryos. Only transplants that included middorsal mesoderm gave rise to lymphocytes.

Published
1984
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16. Automated fluorescent analysis for cytotoxicity assays.

Author

Horan PK and Kappler JW

Subjects
Animals, Autoanalysis, Cell Nucleus immunology, Cytotoxicity Tests, Immunologic, Guinea Pigs, Mice, Rabbits, Spleen immunology, Staining and Labeling, T-Lymphocytes immunology, Trypan Blue, Fluorescent Antibody Technique
Abstract

Classical measurements of cytotoxicity using dye exclusion and microscopic evaluation are both time-consuming and inaccurate. Using a cell sorter (TPS) a single dye system has been developed which stains live and complement killed cells with different fluorescence intensity. After exposure of target cells to antibody and complement, ethidium bromide is added to the target cells at a high enough concentration to stain complement killed cells very intensely. The cells are then diluted and lysed to produce single nuclei, permitting live cells to be stained but less intensely than the dead cells. Fluorescence intensity is measured on single nuclei at a rate of 10,000 per minute. For these studies anti-T antisera was titrated for complement dependent cytotoxic activity using normal mouse spleen cells, spleen cells from an anti-thymocyte serum treated mouse, and nylon wool purified mouse splenic T-cells. This procedure makes possible, reliable and reproducible measurement of cytotoxic activity on 5,000 cells per determination.

Published
1977
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17. Present status of MA-160 cell line. Prostatic epithelium or HeLa cells.

Author

Webber MM, Horan PK, and Bouldin TR

Subjects
Adenoma enzymology, Chromosomes ultrastructure, DNA, Neoplasm metabolism, Epithelial Cells, Epithelium ultrastructure, HeLa Cells, Humans, Male, Middle Aged, Cell Line, Prostate pathology, Prostate ultrastructure, Prostatic Hyperplasia pathology
Abstract

This report reviews the background and the present status of the MA-160 cell line. This cell line was reported to have arisen from tissue cultures of a human, benign prostatic adenoma and consequently has been used for investigations on the prostat and on hormone-dependent cells. Recent studies using chromosome analysis by banding techniques, glucose-6-phosphate dehydrogenase (G6D) electrophoretic mobility, and a specific prostatic acid phosphatase test indicate that MA-160 is not of prostatic origin but a HeLa cell contaminant, arising as a result of intraspecies cell contamination. It is suggested that whenever spontaneous transformation is observed in vitro and established cell lines are being used in the laboratory, the cells in question be thoroughly checked with the currently available chromosomal, biochemical, and cytochemical methods in order to establish their origin and to rule out interspecies and intraspecies cell contamination.

Published
1977

18. Heterogeneity and clonal variation related to cell surface expression of a mouse lung tumor-associated antigen quantified using flow cytometry.

Author

Bahler DW, Lord EM, Kennel SJ, and Horan PK

Subjects
Animals, Antibodies, Monoclonal, Cell Cycle, Cell Line, Cell Membrane immunology, Clone Cells, Flow Cytometry, Fluorescent Antibody Technique, Kinetics, Mice, Mice, Inbred BALB C, Molecular Weight, Antigens, Neoplasm analysis, Antigens, Surface analysis, Lung Neoplasms immunology
Abstract

Previous reports have established that line 1, a spontaneous BALB/c lung carcinoma, expresses a Mr 180,000 tumor-associated surface antigen (TSP-180). In this study, using a monoclonal antibody and flow cytometry to quantify cell surface TSP-180 expression, we found that essentially all cells in a tissue culture-adapted line 1 population express TSP-180, but that the amount of TSP-180 expressed by cells is quite heterogeneous. Variation in amount of TSP-180 was found to be in part related to cell size heterogeneity, and to the expression of TSP-180 being cell cycle-dependent. The amount of surface-expressed TSP-180 correlated somewhat with cell size, and was greater on the average for cells in the G2 cell cycle compartment. However, cells of a defined size and specific cell cycle stage still showed marked heterogeneity of expression. Even though the average amount of TSP-180 expressed per cell decreased during in vitro propagation, little change in heterogeneity was observed. To explore whether any TSP-180-related heterogeneity resulted from heritable variation of expression, 263 limiting dilution-derived line 1 clones were analyzed. The majority displayed, shortly after cloning, heterogeneous TSP-180 profiles and mean TSP-180 levels similar to those observed for the parent tumor. Occasionally, however, clones were isolated that again appeared as heterogeneous as the parent, but differed by as much as 3-fold in mean TSP-180 expression. Extensive passage did not substantially increase the low probability of isolating clones which differed in expression of TSP-180. Differences in TSP-180 expression among clones were found to be relatively stable upon passage, typically maintained after recloning, and large enough to influence clonal susceptibility to TSP-180-directed antibody and complement-mediated lysis. Heritable variation in TSP-180 expression among some clones was also shown to be independent of differences related to cell size, cell cycle, or expression of another line 1 surface antigen (P-100). We concluded that although clones demonstrating large heritable differences in TSP-180 expression can occasionally be isolated, line 1 TSP-180 heterogeneity is predominantly nonheritable, being similar to that present in recently cloned lines, quite stable during in vitro passage, and not totally accounted for by cell cycle or cell size variation.

Published
1984

19. Kinetics of changes in peritoneal cell populations following acute inflammation.

Author

Melnicoff MJ, Horan PK, and Morahan PS

Subjects
Animals, Antibodies, Monoclonal immunology, Cell Count, Cell Movement, Female, Fluorescent Dyes, Kinetics, Macrophages classification, Mice, Mice, Inbred BALB C, Peritonitis chemically induced, Macrophages physiology, Peritoneal Cavity pathology, Peritonitis pathology
Abstract

The kinetics of macrophage (M phi) recruitment to the peritoneum following the induction of acute inflammation by thioglycollate broth (TG) was evaluated after prelabeling resident M phi with the fluorescent cell tracking dye, PKH-1. Most of the PKH-1-labeled resident M phi disappeared from the recoverable peritoneal cell population within the first hour after injection of TG. This disappearance coincided with the inflammatory influx of neutrophils (PMNs) and was sustained for at least 5 days after administration of TG, although the PMN number had returned to resident levels by this time. PKH-1-labeled peritoneal M phi were observed again in most animals at 7 days after injection of TG. The number of labeled M phi recovered at 7 days was approximately twice the number of resident peritoneal M phi in control animals which did not receive the TG broth. These additional M phi may include progeny of either the resident M phi or other local M phi precursors, such as omental M phi, which were labeled by the PKH-1 injection.

Published
1989
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20. Expression of viral antigens after infection of human lymphocytes, monocytes, and macrophages with influenza virus.

Author

Roberts NJ Jr and Horan PK

Subjects
Cell Membrane immunology, Cells, Cultured, Flow Cytometry, Fluorescent Antibody Technique, Hemagglutinins, Viral analysis, Humans, Influenza A virus metabolism, Neuraminidase biosynthesis, Viral Matrix Proteins, Viral Proteins biosynthesis, Antigens, Viral analysis, Influenza A virus immunology, Lymphocytes microbiology, Macrophages microbiology, Monocytes microbiology
Abstract

Previous studies demonstrated that in vitro infection with influenza A viruses altered several functions of human monocytes and macrophages, but did not detectably alter functions of human lymphocytes. For a determination of whether both types of leukocytes can be infected by the influenza viruses, human mononuclear leukocytes were infected in vitro and assayed for newly produced and cell surface-expressed viral antigens, with use of indirect immunofluorescence techniques and flow cytometry. Infected cells, including both monocytes and lymphocytes, expressed viral hemagglutinin, neuraminidase, and matrix protein on their surfaces. The expression of influenza virus antigens by such immunocompetent cells may be important in human antiviral defense.

Published
1985
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21. Flow cytometry: rapid isolation and analysis of single cells.

Author

Jensen BD and Horan PK

Subjects
Animals, Cells analysis, DNA analysis, Enzymes analysis, Flow Cytometry instrumentation, Fluorescent Antibody Technique, Fluorescent Dyes, Indicators and Reagents, Proteins analysis, RNA analysis, Spectrometry, Fluorescence instrumentation, Spectrometry, Fluorescence methods, Cell Separation methods, Cells cytology, Flow Cytometry methods
Published
1989
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23. Flow cytometric analysis of blood cells stained with the cyanine dye DiOC1[3]: reticulocyte quantification.

Author

Jacobberger JW, Horan PK, and Hare JD

Subjects
Animals, Erythrocyte Aging, Erythrocyte Count methods, Erythrocytes cytology, Female, Flow Cytometry methods, Fluorescent Dyes, Mice, Mice, Inbred BALB C, Rats, Rats, Inbred Strains, Reticulocytes cytology
Abstract

The fluorescent dye 3,3'-dimethyloxacarbocyanine (DiOC1[3]) is taken up by all cells in mammalian blood which then fluoresce as follows: mature erythrocytes less than immature erythrocytes congruent to platelets less than leukocytes. A continuous fluorescence distribution can be generated for the red blood cells by flow cytometry and deconvolved into two arbitrary populations, mature and immature erythrocytes (mRBC and imRBC). This analysis mimics the established method of counting imRBC stained with the supravital dyes, new methylene blue, brilliant cresyl blue (BCB), and acridine orange (AO). However, the population of imRBC as quantified by DiOC1[3] fluorescence is a subset of reticulocytes (reticulocytes as determined by BCB assay). The advantages and disadvantages of using DiOC1[3], AO, or pyronine Y as reticulocyte stains are discussed.

Published
1984
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24. Improved flow cytometric analysis of leukocyte subsets: simultaneous identification of five cell subsets using two-color immunofluorescence.

Author

Horan PK, Slezak SE, and Poste G

Subjects
Antibodies, Monoclonal immunology, Color, Fluorescent Antibody Technique, Humans, Leukocytes immunology, Lymphocytes classification, Flow Cytometry, Leukocytes classification
Abstract

Flow cytometric analysis of human peripheral blood leukocytes has typically been achieved by staining multiple aliquots of the same sample with fluorescent reagents specific for cell subsets of interest. Spectrally discrete fluorochrome tags have been developed for applications in which identification of multiple subsets (e.g., T and B cells) or of subsets not uniquely identified by a single reagent (e.g., activated T cells) requires use of multiple reagents per aliquot. Extension of this approach to more than two reagents per aliquot has led to multicolor methods requiring dual laser excitation and complex instrumentation. We describe an alternative two-color method using commercially available reagents that allows simultaneous identification of five discrete immune cell subsets using only a single excitation source. The technique uses dilution of commercial fluorochrome-labeled reagents with competing unlabeled reagents to selectively produce discrete fluorescence intensity profiles for cell subsets that would otherwise display overlapping or indistinguishable profiles when stained with reagents bearing the same fluorochrome. For example, the fluorescence intensity of phycoerythrin-labeled helper T (Th) cells can be adjusted to be distinct from that of phycoerythrin-labeled suppressor T (Ts) cells. Extending this technique to two colors, we have used a combination of seven different monoclonal antibodies to simultaneously quantify Th, Ts, B cells, natural killer cells, and monocytes in a single aliquot. An additional advantage of this approach is the ability to more accurately quantify "null" cells. Adjustment of fluorescence intensity profiles of different cell subsets by this method is applicable to flow cytometric analysis of a wide variety of cell types. The technique significantly extends the analytical capacity of flow cytometry without significantly increasing the complexity of the instrumentation required.

Published
1986
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25. Stable cell membrane labelling.

Author

Horan PK and Slezak SE

Subjects
Animals, Biomarkers, Cell Movement, Microscopy, Fluorescence, Spectrometry, Fluorescence, Cell Membrane metabolism, Fluorescent Dyes, Lipid Bilayers metabolism, Molecular Probe Techniques
Abstract

Binding fluorescent or radioactive reporter molecules to the lipid bilayer of cell membranes allows cell growth and trafficking to be monitored in vivo.

Published
1989
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26. Quantitative single cell analysis and sorting.

Author

Horan PK and Wheeless LL Jr

Subjects
Antibiotics, Antineoplastic therapeutic use, Binding Sites, Cell Division, DNA analysis, DNA, Neoplasm analysis, Electricity, Klinefelter Syndrome diagnosis, Lymphocytes immunology, Neoplasms diagnosis, Neoplasms drug therapy, Neoplasms pathology, Rheology, Spectrometry, Fluorescence, Cell Separation instrumentation
Published
1977
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27. Improved detection of rare CALLA-positive cells in peripheral blood using multiparameter flow cytometry.

Author

Ryan DH, Mitchell SJ, Hennessy LA, Bauer KD, Horan PK, and Cohen HJ

Subjects
Adult, Bone Marrow immunology, Clinical Laboratory Techniques, Flow Cytometry methods, Fluorescent Antibody Technique, Humans, Neprilysin, Reference Values, Antigens, Neoplasm analysis, Leukemia, Lymphoid immunology
Abstract

A major limitation to the detection of rare cell types in the peripheral blood using monoclonal antibodies is nonspecific binding of the antibody reagent to normal cells. Detection of rare common acute lymphoblastic leukemia antigen (CALLA)-positive cells in peripheral blood is significantly improved by using multiple flow cytometric parameters to exclude a variety of mature blood cells which may nonspecifically bind the antibody reagent. Monocytes and granulocytes are excluded by gating out cells with high 90 degrees light scatter. By gating on red fluorescence, a variety of mature cell types binding to phycoerythrin (PE)-conjugated Leu 3, Leu 2, and M3 monoclonal antibodies are also excluded. CALLA-positive lymphoblasts from 6 consecutive patients were not excluded on the basis of these parameters. Gating on log 90 degrees light scatter and log red fluorescence in this fashion reduced the incidence of nonspecific binding to peripheral blood mononuclear cells of a fluorescein-conjugated irrelevant monoclonal antibody by 98% from 308 cells per million to 5 cells per million. One CALLA-positive lymphoblast per 100,000 peripheral blood mononuclear cells could be detected in mixture experiments using this method. The normal range of CALLA-positive cells in adults is less than 16 cells per million peripheral blood mononuclear cells. This low background of CALLA-positive peripheral blood cells may permit the detection of early leukemic relapse in acute lymphoblastic leukemia by analysis of the peripheral blood. This methodology can be applied to the detection of any rare cell type by using phycoerythrin-conjugated antibodies to markers that the cell type does not possess.

Published
1984
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30. Methodological considerations for implementation of lymphocyte subset analysis in a clinical reference laboratory.

Author

Muirhead KA, Wallace PK, Schmitt TC, Frescatore RL, Franco JA, and Horan PK

Subjects
Antibodies, Monoclonal analysis, Blood Specimen Collection, Flow Cytometry, Fluorescent Antibody Technique, Hemolysis, Humans, Reference Values, Laboratories, Lymphocytes cytology
Abstract

As the diagnostic utility of lymphocyte subset analysis has been recognized in the clinical research laboratory, a wide variety of reagents and cell preparation, staining and analysis methods have also been described. Methods that are perfectly suitable for analysis of smaller sample numbers in the biological or clinical research setting are not always appropriate and/or applicable in the setting of a high volume clinical reference laboratory. We describe here some of the specific considerations involved in choosing a method for flow cytometric analysis which minimizes sample preparation and data analysis time while maximizing sample stability, viability, and reproducibility. Monoclonal T- and B-cell reagents from three manufacturers were found to give equivalent results for a reference population of healthy individuals. This was true whether direct or indirect immunofluorescence staining was used and whether cells were prepared by Ficoll-Hypaque fractionation (FH) or by lysis of whole blood. When B cells were enumerated using a polyclonal anti-immunoglobulin reagent, less cytophilic immunoglobulin staining was present after lysis than after FH preparation. However, both preparation methods required additional incubation at 37 degrees C to obtain results concordant with monoclonal B-cell reagents. Standard reagents were chosen on the basis of maximum positive/negative separation and the availability of appropriate negative controls. The effects of collection medium and storage conditions on sample stability and reproducibility of subset analysis were also assessed. Specimens collected in heparin and stored at room temperature in buffered medium gave reproducible results for 3 days after specimen collection, using either FH or lysis as the preparation method. General strategies for instrument optimization, quality control, and biohazard containment are also discussed.

Published
1986
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31. Antitumor immunity induced by hybrid tumor cells: comparison between hybrids and the parental tumor.

Author

O'Donnell RW, Horan PK, Minken TJ, Chuang C, Henshaw EC, and McCune CS

Subjects
Animals, Cell Line, Female, Immunity, Cellular, Mice, Mice, Inbred BALB C, Mice, Inbred C3H, Propionibacterium acnes immunology, Adenocarcinoma, Bronchiolo-Alveolar immunology, Hybrid Cells immunology, Lung Neoplasms immunology
Abstract

The ability of hybrid tumor cells to induce antitumor immunity has been evaluated in the line 1 alveolar cell carcinoma (L1) model of BALB/c mice. Hybrid tumor cells were produced by fusing freshly dissociated L1 cells isolated from in vivo tumors with the hypoxanthine:aminopterin:thymidine-sensitive cell line, GM 347, derived from C3H mice. Each hybrid was characterized by DNA content and expression of H-2 antigens using a fluorescence-activated cell sorter. Irradiated L1 cells in the presence or absence of Corynebacterium parvum were capable of immunizing BALB/c mice against a challenge of live L1 cells, provided the challenge dose was small (50% lethal dose was between 6 X 10(4) and 1.2 X 10(5) L1 cells). Testing of five hybrid clones and 1 uncloned hybrid line for their immunizing ability demonstrated a range in immunizing ability with none showing a statistically significant improvement in survival (p less than 0.0018) when compared to untreated controls. However, one hybrid clone, MoHb-L1-C2, was selected in which the survival of mice immunized with it compared to controls had a p value of 0.0255. A tumor (labeled L1/A) which grew in one of the mice immunized with this clone was removed and hybridized with GM 347 to yield a second set of hybrids. Both this variant of L1 cells and a hybrid clone made from it (MoHb-L1A-C18) were capable of immunizing mice against a challenge of live L1/A (p values of 0.0000 and 0.0028, respectively, when compared to controls). However, L1 cells were not able to immunize effectively against L1/A, and MoHb-L1A-C18 did not immunize against L1. This suggests that L1/A is a subpopulation of L1 cells with a different antigenic composition. The limited success of MoHb-L1A-C18 against L1/A is thought to be due to the narrower range of antigenic specificities in L1/A and the ability of MoHb-L1A-C18 to represent an important antigenic subpopulation of L1/A.

Published
1984

32. A comparison of acridine orange and Feulgen cytochemistry of human tumor cell nuclei.

Author

Gill JE, Wheeless LL Jr, Hanna-Madden C, Marisa RJ, and Horan PK

Subjects
Animals, Cell Nucleus metabolism, DNA metabolism, Female, Histocytochemistry, Humans, Liver metabolism, Rats, Spectrometry, Fluorescence, Acridines metabolism, DNA, Neoplasm metabolism, Genital Neoplasms, Female metabolism, Staining and Labeling
Abstract

Specimens of cells derived from tumors of the human female genital tract plus normal cells as standards have been divided into aliquots and stained according to acridine orange or pararosanilin:Feulgen procedures. Acridine orange-stained cells were slit-scanned for 535 nm nuclear fluorescence; Feulgen-stained cells were comb-scanned for 580 nm nuclear absorbance. For each specimen examined, the tumor cell:normal cell ratio of mean nuclear fluorescence following acridine orange staining was greater than the tumor cell:normal cell ratio of mean nuclear absorbance following Feulgen staining. The tumor cell:normal cell ratio of mean nuclear fluorescence ranged from 2.3 for a nonkeratinizing squamous cell carcinoma to 3.9 for a keratinizing squamous cell carcinoma. The tumor cell:normal cell ratio of mean nuclear absorbance ranged from 1.4 for a mixed mesodermal sarcoma to 2.3 for a small cell squamous cell carcinoma. These results indicate that the elevated nuclear fluorescence intensity from acridine orange-stained tumor cells cannot be explained solely on the basis of elevated Feulgen:DNA content. An alternative hypothesis, consistent with these results, is that DNA is the principal binding substrate for intranuclear acridine orange and that the DNA of certain tumor cells is more accessible to acridine orange than is the DNA of normal cells.

Published
1978

33. A cyanine dye distinguishes between cycling and non-cycling fibroblasts.

Author

Cohen RL, Muirhead KA, Gill JE, Waggoner AS, and Horan PK

Subjects
Cell Survival drug effects, Cells, Cultured, Cytoplasm physiology, Humans, Membrane Potentials, Carbocyanines, Cell Division, Fibroblasts cytology, Fluorescent Dyes pharmacology, Quinolines
Abstract

Cellular proliferative activity has previously been determined by measuring the incorporation of radiolabelled nucleotides or by visual inspection of cellular morphology. Although two flow cytometric methods have recently been developed which can distinguish cycling from non-cycling cells, both have serious disadvantages. One method requires uptake of a substantial amount of BUdR, limiting its usefulness for in vitro systems. The other method utilizes RNA/DNA content differences but its successful application has proved cell-type dependent. We have now used the findings that the cell membrane is more highly polarized in resting than in proliferating cells and that cyanine dyes carrying a delocalized positive charge enter live cells to an extent that depends on the cell membrane potential, to develop a method of distinguishing between cycling and non-cycling cells. The greater the membrane polarization, the greater is the concentration of dye within the cell. At high concentrations, the dye molecules aggregate and their fluorescence is quenched. Thus, for a given external dye concentration, cells of different membrane potential would accumulate different amounts of fluorescent (non-aggregated) dye. Using fibroblasts in culture conditions chosen to provide various models of cycling and non-cycling cells, we found that fluorescence intensity with the dye, 3,3'-diheptyloxycarbocyanine (Di-O-C,(3)) was consistently greater in the former than the latter.

Published
1981
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35. Aseptic aspiration of rabbit bone marrow and enrichment for cycling cells.

Author

Horan PK, Muirhead KA, Gorton S, and Irons RD

Subjects
Animals, Biopsy, Needle instrumentation, Biopsy, Needle methods, Cell Separation, Female, Femur cytology, Humerus cytology, Biopsy, Needle veterinary, Bone Marrow Cells, Rabbits anatomy & histology
Abstract

Female adult New Zealand white rabbits were anesthetized using a combination of xylazine and ketamine administered intramuscularly. Bone marrow was aspirated aseptically from the humerus of femur using an 18-gauge Rosenthal pediatric needle. Marrow was obtained from six animals per hour using this technique. Recovery was rapid and no infection or loss of limb function was observed over the course of more than 100 aspirations. Approximately 2 x 10(8) mononuclear cells were obtained from 0.5 ml of aspirated marrow. Marrow samples were fractioned using isopynic single step density gradients. A 10-fold enrichment of blast cells was achieved using a density of 1.077 g/ml.

Published
1980

37. Syringing as a method of cell dispersal. I. Effect on intermediate and superficial squamous cells.

Author

Mead JS, Horan PK, and Wheeless LL Jr

Subjects
Cell Separation instrumentation, Female, Humans, Syringes, Cell Separation methods, Specimen Handling methods, Vaginal Smears
Abstract

Mechanical shear in the form of syringing was applied to human gynecologic cytology specimens in an effort to disperse cell clumps. The percentage of single squamous cells achieved with the optimum conditions is generally 70 to 100 per cent. Syringing with a constant pressure device produces a high yield of single squamous cells without the concurrent high cell loss as often observed using enzymatic or chemical procedures. Data presented demonstrate that the slide preparation and clump evaluation procedures used for this study yield reliable and reproducible data. Studies varying stroke number and plunger pressure were completed and conditions for maximum dispersal were established.

Published
1978

38. A rabbit bone marrow model system for evaluation of cytotoxicity: characterization of normal bone marrow cell cycle parameters by flow cytometry.

Author

Muirhead KA, Irons RD, Bruns R, and Horan PK

Subjects
Animals, Cell Cycle, DNA analysis, Female, Histocytochemistry, Rabbits, Bone Marrow physiology, Drug Evaluation, Preclinical methods
Abstract

Characterization of a rabbit model system for the study of cell cycle effects of myelotoxic agents in normal bone marrow is described. Cell cycle phase distributions are obtained by computer analysis of flow cytometric single cell DNA histograms. Comparison of marrow aspirates with marrow samples from sacrificed animals indicates that dilution of aspirates with peripheral blood is not significant. Aspiration of marrow from one bone does not affect the cell cycle distribution of unsampled bones. Hence, sequential aspirates of different bones in a single animal may be used as representative samples for further study of effects of myelotoxins on marrow proliferation and differentiation.

Published
1980
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39. In vivo labeling of resident peritoneal macrophages.

Author

Melnicoff MJ, Morahan PS, Jensen BD, Breslin EW, and Horan PK

Subjects
Animals, Antibodies, Monoclonal, Antigens, Surface analysis, Flow Cytometry methods, Fluorescent Antibody Technique, Fluorescent Dyes, Inflammation pathology, Lasers, Mice, Rats, Solubility, Macrophages cytology, Peritoneum cytology, Phagocytes cytology
Abstract

A novel method for labeling resident peritoneal macrophages (M phi) by injection of a dye into the peritoneal cavity is described. The dye, which fluoresces green, is selectively taken up by the resident M phi. Dye labeled cells can be further characterized by labeling of cell surface antigens with monoclonal antibodies (Mabs) and phycoerythrin conjugated second antibody. After such labeling with the Mabs F4/80 or Mac 1 the resident M phi were labeled by both the green dye and the red Mab markers, while recruited M phi or neutrophils were labeled with just the red Mab; the two populations of cells were readily distinguished by two-color flow cytometry. This technique enabled identification of resident and recruited M phi in each animal without the use of radioisotopes, irradiation, or bone marrow ablation. Sufficient numbers of cells can be analyzed from each animal so that individual animals could be evaluated. We found no adverse effects of this labeling technique on expression of cell surface antigens or M phi mediated cytotoxicity. We did find evidence that the i.p. injection induced a mild inflammation in the peritoneal cavities of animals injected with either the dye or the balanced salt solution vehicle. Examination of the intracellular staining pattern indicated that the label rapidly sequestered in the cytoplasm of the M phi, possibly in the lysosomes. Dye solubility studies showed that the dye was partially soluble at the concentration used for in vivo labeling. We hypothesize that the M phi labeling occurred by a combination of phagocytosis of dye aggregates and endocytosis of labeled plasma membrane.

Published
1988
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40. A strain of Escherichia coli with minimum postirradiation degradation properties.

Author

Horan PK, Hird K, and Pollard EC

Subjects
Cobalt Isotopes, Coliphages radiation effects, Culture Media, DNA Repair, DNA, Bacterial analysis, DNA, Bacterial biosynthesis, DNA, Single-Stranded, Escherichia coli growth & development, Escherichia coli metabolism, Mutation, RNA, Bacterial biosynthesis, Ultraviolet Rays, DNA, Bacterial radiation effects, Escherichia coli radiation effects, Radiation Effects
Published
1972

42. Multiparameter analysis and sorting of mammalian cells.

Author

Steinkamp JA, Romero A, Horan PK, and Crissman HA

Subjects
Acridines, Animals, Autoradiography, Cell Line, Cricetinae, Cytological Techniques instrumentation, DNA biosynthesis, Dogs, Female, Fluorescent Dyes, HeLa Cells, Humans, Leukocytes, Lymphocytes, Mice, Neoplasms, Experimental, Ovary, Spleen, Staining and Labeling, Thymidine metabolism, Tritium, Cell Separation
Published
1974
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43. Detection of heteroploid tumor cells.

Author

Horan PK, Romero A, Steinkamp JA, and Petersen DF

Subjects
Animals, Carcinoma, Squamous Cell chemically induced, Cells, Cultured, Fluorometry, Methods, Methylcholanthrene, Mice, Mice, Inbred C3H, Neoplasm Transplantation, Neoplasms, Experimental chemically induced, Neoplasms, Experimental diagnosis, Transplantation, Homologous, Carcinoma, Squamous Cell diagnosis, Cytodiagnosis, DNA, Neoplasm analysis
Published
1974
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45. Free-radical production by heavy ions at 77 degrees-K and its relation to the thermal spike theory.

Author

Henriksen T, Horan PK, and Snipes W

Subjects
Argon, Carbon, Cysteine radiation effects, Electron Spin Resonance Spectroscopy, Electrons, Energy Transfer, Free Radicals, Helium, Ions, Muramidase radiation effects, Neon, Pepsin A radiation effects, Ribonucleases radiation effects, Threonine radiation effects, Valine radiation effects, Amino Acids radiation effects, Hot Temperature, Proteins radiation effects, Radiation Effects, Radiochemistry
Published
1970

50. Stability of radiation-induced organic free radicals. Decay by heat.

Author

Horan PK, Taylor WD, Strother GK, and Snipes W

Subjects
Alanine analysis, Amino Acids analysis, Electric Conductivity, Electron Spin Resonance Spectroscopy, Electrons, Free Radicals, Ions, Kinetics, Spectrum Analysis, Tartrates analysis, Valine analysis, Hot Temperature, Radiochemistry
Abstract

The rate of free radical decay was measured at various temperatures using electron paramagnetic resonance spectroscopy. Rate constants determined from first-order decay kinetics were used to determine the activation energy for the process of free radical decay. The similarity between the temperature dependence of free radical decay by heat and that of electrical conductivity has led us to consider the possibility that the two processes may be related. Mechanisms by which a population of electron-hole conducting states may lead to free radical decay are outlined and experimental data relating to these mechanisms are discussed.

Published
1968
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