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1. Characterisation of newly isolated genes expressed in the ovary of Drosophila melanogaster

Author

Grimes, Brenda R.

Subjects
591.35
Abstract

Two genomic clones called λov5 and λov2 were isolated from a differential screen and found to encode ovary enriched transcripts. The genes within λov2 and λov5 have been initially characterised with a view to ultimately determining their function(s) during oogenesis. λ0v5 consists of two EcoRI sub-fragments denoted ov5A and ov5B. Each of these fragments detect ovary enriched transcripts on Northern blots. The ov5A probe was used to screen a λgt11 ovary cDNA library and three size classes of cDNA called λov5A1, λov5A2 and λov5A5 were identified. Each cDNA detects at least two ovary enriched transcripts, approximately 1.7 kb and 1.4 kb in length. The ov5A5 cDNA also hybridises with two additional ovary specific transcripts approximately 0.8 kb and 0.2 kb in length. The organisation of these ovary transcripts within the ov5A genomic region was determined by cross-hybridisation of cDNAs to Southern blots of restriction enzyme digests of ov5A sequences. The ov5B sub-fragment detects an ovary specific transcript approximately 1.4 kb in length. Full length cDNA copies of this transcript were isolated. In situ hybridisation to whole mounts of Drosophila ovaries were carried out using digoxigenin-labelled ov5A2 and ov5B1 cDNA probes to determine the spatial and temporal distribution of the ovary enriched transcripts during oogenesis. ov5A2 detects transcripts in the nurse cell cytoplasm and in oocytes from stage 7 onwards. ov5B1 strongly detects transcripts in stage 10B nurse cell cytoplasm and in the degenerating nurse cells. Two EcoRI sub-fragments of λov2, ov2A and ov2B, hybridise with female cDNA but not with male cDNA. ov2A detects two ovary and embryo specific transcripts approximately 4.0 kb and 3.0 kb in size and also a 1.6 kb sized male-specific transcript. ov2B detects two transcripts estimated to be 3.5 kb and 2.5 kb in length which are expressed exclusively in the ovary. λov5 and λov2 were mapped on chromosome 3R at positions 88B/C and 89B respectively. Within the cytological region 88-89, two female sterile mutations called Spindle-B and fs293gamma5 have been genetically mapped. Experiments with a set of deficiency chromosomes were carried out to determine whether or not the ov5 or ov2 genomic sequences mapped close to these mutations.

Published
1990

4. Adjuvant Abemaciclib Combined with Endocrine Therapy: Efficacy Results in monarchE Cohort 1.

Author

Toi, Masakazu, Boyle, Frances, Im, Young-Hyuck, Reinisch, Mattea, Molthrop, David, Jiang, Zefei, Wei, Ran, Sapunar, Francisco, Grimes, Brenda R, Nabinger, Sarah Cassidy, and Johnston, Stephen R D

Subjects
THERAPEUTIC use of antineoplastic agents, ADJUVANT chemotherapy, HORMONE therapy, CONFIDENCE intervals, CANCER relapse, ANTINEOPLASTIC agents, TREATMENT effectiveness, DESCRIPTIVE statistics, RESEARCH funding, STATISTICAL sampling, ODDS ratio, BREAST tumors, PATIENT safety
Abstract

The monarchE Cohort 1 patient population was enrolled based on high-risk clinicopathological features that can easily be identified as part of routine clinical breast cancer evaluation. Efficacy data from Cohort 1 demonstrate substantial evidence of benefit for adjuvant abemaciclib+ET in patients with HR+, HER2− early breast cancer at high risk of recurrence (ClinicalTrials.gov: NCT03155997 [monarchE]). [ABSTRACT FROM AUTHOR]

Published
2023
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7. A real-world US study of recurrence risks using combined clinicopathological features in HR-positive, HER2-negative early breast cancer.

Author

Sheffield, Kristin M, Peachey, Jessica R, Method, Michael, Grimes, Brenda R, Brown, Jacqueline, Saverno, Kim, Sugihara, Tomoko, Cui, Zhanglin Lin, and Lee, Kimberley T

Subjects
PROGNOSIS, CANCER relapse, CELL receptors, BREAST tumors, PROPORTIONAL hazards models
Abstract

Aim: To assess invasive disease-free survival (IDFS) and distant relapse-free survival (DRFS) in hormone receptor-positive, HER2-negative early breast cancer with combined clinicopathological criteria from monarchE, a phase III study of abemaciclib. Methods: US electronic health records were used to compare outcomes between high-risk (≥4 lymph nodes, or 1-3 lymph nodes and grade 3, tumor ≥5 cm or Ki-67 ≥20%) versus nonhigh-risk groups using Kaplan-Meier methods and Cox regression models. Results: The high-risk group (n = 557) was at higher risk for IDFS and DRFS events than the nonhigh-risk group (n = 3471). IDFS events (hazard ratio: 3.07; 95% CI: 2.45-3.83) and DRFS events (hazard ratio: 3.15; 95% CI: 2.49-3.97) were significantly higher for the high-risk group. Conclusion: Risk of recurrence was three-times greater in the high-risk group, highlighting the need for better therapies. [ABSTRACT FROM AUTHOR]

Published
2022
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11. Phenotypic plasticity in normal breast derived epithelial cells.

Author

Sauder, Candice A. M., Koziel, Jillian E., MiRan Choi, Fox, Melanie J., Grimes, Brenda R., Badve, Sunil, Blosser, Rachel J., Radovich, Milan, Lam, Christina C., Vaughan, Melville B., Herbert, Brittney-Shea, and Clare, Susan E.

Subjects
MATERIAL plasticity, BREAST, METAPLASIA, SQUAMOUS cell carcinoma, EMBRYOLOGY
Abstract

Background Normal, healthy human breast tissue from a variety of volunteer donors has become available for research thanks to the establishment of the Susan G. Komen for the Cure® Tissue Bank at the IU Simon Cancer Center (KTB). Multiple epithelial (K-HME) and stromal cells (K-HMS) were established from the donated tissue. Explant culture was utilized to isolate the cells from pieces of breast tissue. Selective media and trypsinization were employed to select either epithelial cells or stromal cells. The primary, non-transformed epithelial cells, the focus of this study, were characterized by immunohistochemistry, flow cytometry, and in vitro cell culture. Results All of the primary, non-transformed epithelial cells tested have the ability to differentiate in vitro into a variety of cell types when plated in or on biologic matrices. Cells identified include stratified squamous epithelial, osteoclasts, chondrocytes, adipocytes, neural progenitors/neurons, immature muscle and melanocytes. The cells also express markers of embryonic stem cells. Conclusions The cell culture conditions employed select an epithelial cell that is pluri/multipotent. The plasticity of the epithelial cells developed mimics that seen in metaplastic carcinoma of the breast (MCB), a subtype of triple negative breast cancer; and may provide clues to the origin of this particularly aggressive type of breast cancer. The KTB is a unique biorepository, and the normal breast epithelial cells isolated from donated tissue have significant potential as new research tools. [ABSTRACT FROM AUTHOR]

Published
2014
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12. A new assay for measuring chromosome instability (CIN) and identification of drugs that elevate CIN in cancer cells.

Author

Hee-Sheung Lee, Lee, Nicholas C. O., Grimes, Brenda R., Samoshkin, Alexander, Kononenko, Artem V., Bansal, Ruchi, Masumoto, Hiroshi, Earnshaw, William C., Kouprina, Natalay, and Larionov, Vladimir

Subjects
ANEUPLOIDY, CANCER cells, CHROMOSOME abnormalities, CANCER invasiveness, ARTIFICIAL chromosomes, FLOW cytometry
Abstract

Background: Aneuploidy is a feature of most cancer cells that is often accompanied by an elevated rate of chromosome mis-segregation termed chromosome instability (CIN). While CIN can act as a driver of cancer genome evolution and tumor progression, recent findings point to the existence of a threshold level beyond which CIN becomes a barrier to tumor growth and therefore can be exploited therapeutically. Drugs known to increase CIN beyond the therapeutic threshold are currently few in number, and the clinical promise of targeting the CIN phenotype warrants new screening efforts. However, none of the existing methods, including the in vitro micronuclei (MNi) assay, developed to quantify CIN, is entirely satisfactory. Methods: We have developed a new assay for measuring CIN. This quantitative assay for chromosome missegregation is based on the use of a non-essential human artificial chromosome (HAC) carrying a constitutively expressed EGFP transgene. Thus, cells that inherit the HAC display green fluorescence, while cells lacking the HAC do not. This allows the measurement of HAC loss rate by routine flow cytometry. Results: Using the HAC-based chromosome loss assay, we have analyzed several well-known anti-mitotic, spindletargeting compounds, all of which have been reported to induce micronuclei formation and chromosome loss. For each drug, the rate of HAC loss was accurately measured by flow cytometry as a proportion of non-fluorescent cells in the cell population which was verified by FISH analysis. Based on our estimates, despite their similar cytotoxicity, the analyzed drugs affect the rates of HAC mis-segregation during mitotic divisions differently. The highest rate of HAC mis-segregation was observed for the microtubule-stabilizing drugs, taxol and peloruside A. Conclusion: Thus, this new and simple assay allows for a quick and efficient screen of hundreds of drugs to identify those affecting chromosome mis-segregation. It also allows ranking of compounds with the same or similar mechanism of action based on their effect on the rate of chromosome loss. The identification of new compounds that increase chromosome mis-segregation rates should expedite the development of new therapeutic strategies to target the CIN phenotype in cancer cells. [ABSTRACT FROM AUTHOR]

Published
2013
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13. A Telomerase Immortalized Human Proximal Tubule Cell Line with a Truncation Mutation (Q4004X) in Polycystin-1.

Author

Herbert, Brittney-Shea, Grimes, Brenda R., Wei Min Xu, Werner, Michael, Ward, Christopher, Rossetti, Sandro, Harris, Peter, Bello-Reuss, Elsa, Ward, Heather H., Miller, Caroline, Gattone II, Vincent H., Phillips, Carrie L., Wandinger-Ness, Angela, and Bacallao, Robert L.

Subjects
*POLYCYSTIC kidney disease, *EPITHELIAL cells, *CELL culture, *CELL lines, *NEPHRONS, *CYSTS (Pathology)
Abstract

Autosomal dominant polycystic kidney disease (ADPKD) is associated with a variety of cellular phenotypes in renal epithelial cells. Cystic epithelia are secretory as opposed to absorptive, have higher proliferation rates in cell culture and have some characteristics of epithelial to mesenchymal transitions [1,2]. In this communication we describe a telomerase immortalized cell line that expresses proximal tubule markers and is derived from renal cysts of an ADPKD kidney. These cells have a single detectable truncating mutation (Q4004X) in polycystin-1. These cells make normal appearing but shorter cilia and fail to assemble polycystin-1 in the cilia, and less uncleaved polycystin-1 in membrane fractions. This cell line has been maintained in continuous passage for over 35 passages without going into senescence. Nephron segment specific markers suggest a proximal tubule origin for these cells and the cell line will be useful to study mechanistic details of cyst formation in proximal tubule cells. [ABSTRACT FROM AUTHOR]

Published
2013
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14. Human umbilical cord blood plasma can replace fetal bovine serum for in vitro expansion of functional human endothelial colony-forming cells.

Author

Lan Huang, Critser, Paul J., Grimes, Brenda R., and Yoder, Mervin C.

Subjects
CELL proliferation, BLOOD vessels, CORD blood, CELL culture, CYTOKINES
Abstract

Background aims. A hierarchy of endothelial colony-forming cells (ECFC) with different levels of proliferative potential has been identified in human circulating blood and blood vessels. ECFC has recently become an attractive target for new vascular regenerative therapies; however, in vitro expansion of ECFC typically depends on the presence of fetal bovine serum (FBS) or fetal calf serum (FCS) in the culture medium, which is not appropriate for its therapeutic application. Methods. To identify optimal conditions for in vitro expansion of ECFC, the effects of human endothelial serum-free medium (SFM) supplemented with six pro-angiogenic cytokines and human umbilical cord blood plasma (HCP) were investigated. The in vitro morphology, proliferation, surface antigen expression and in vivo vessel-forming ability were utilized for examining the effects of medium on ECFC. Results. This novel formulation of endothelial cell culture medium allows us, for the first time, to isolate and expand human ECFC efficiently in vitro with a low concentration of HCP (1.5%) and without bovine serum additives. In this serum-reduced medium (SRM), human ECFC colony yields remained quantitatively similar to those cultured in a high concentration (10%) of bovine serum-supplemented medium. SRM-cultured ECFC displayed a robust clonal proliferative ability in vitro and human vessel-forming capacity in vivo. Conclusions. The present study provides a novel method for the expansion of human ECFC in vitro and will help to advance approaches for using the cells in human therapeutic trials. [ABSTRACT FROM AUTHOR]

Published
2011
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15. α-Satellite DNA and Vector Composition Influence Rates of Human Artificial Chromosome Formation

Author

Grimes, Brenda R., Rhoades, Angela A., and Willard, Huntington F.

Subjects
*HUMAN chromosomes, *GENETIC transformation, *GENE therapy
Abstract

Human artificial chromosomes (HACs) have been proposed as a new class of potential gene transfer and gene therapy vector. HACs can be formed when bacterial cloning vectors containing α-satellite DNA are transfected into cultured human cells. We have compared the HAC-forming potential of different sequences to identify features critical to the efficiency of the process. Chromosome 17 or 21 α-satellite arrays are highly competent HAC-forming substrates in this assay. In contrast, a Y-chromosome-derived α-satellite sequence is inefficient, suggesting that centromere specification is at least partly dependent on DNA sequence. The length of the input array is also an important determinant, as reduction of the chromosome-17-based array from 80 kb to 35 kb reduced the frequency of HAC formation. In addition to the α-satellite component, vector composition also influenced HAC formation rates, size, and copy number. The data presented here have a significant impact on the design of future HAC vectors that have potential to be developed for therapeutic applications and as tools for investigating human chromosome structure and function. [Copyright &y& Elsevier]

Published
2002
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16. A new assay for measuring chromosome instability (CIN) and identification of drugs that elevate CIN in cancer cells.

Author

Lee, Hee-Sheung, Lee, Nicholas Co, Grimes, Brenda R, Samoshkin, Alexander, Kononenko, Artem V, Bansal, Ruchi, Masumoto, Hiroshi, Earnshaw, William C, Kouprina, Natalay, Larionov, Vladimir, and Lee, Nicholas C O

Subjects
ANTINEOPLASTIC agents, CELL lines, CHROMOSOME abnormalities, CHROMOSOMES, FLOW cytometry, GENES, GENETIC techniques, PROTEINS, FLUORESCENCE in situ hybridization, PHARMACODYNAMICS
Abstract

Background: Aneuploidy is a feature of most cancer cells that is often accompanied by an elevated rate of chromosome mis-segregation termed chromosome instability (CIN). While CIN can act as a driver of cancer genome evolution and tumor progression, recent findings point to the existence of a threshold level beyond which CIN becomes a barrier to tumor growth and therefore can be exploited therapeutically. Drugs known to increase CIN beyond the therapeutic threshold are currently few in number, and the clinical promise of targeting the CIN phenotype warrants new screening efforts. However, none of the existing methods, including the in vitro micronuclei (MNi) assay, developed to quantify CIN, is entirely satisfactory.Methods: We have developed a new assay for measuring CIN. This quantitative assay for chromosome mis-segregation is based on the use of a non-essential human artificial chromosome (HAC) carrying a constitutively expressed EGFP transgene. Thus, cells that inherit the HAC display green fluorescence, while cells lacking the HAC do not. This allows the measurement of HAC loss rate by routine flow cytometry.Results: Using the HAC-based chromosome loss assay, we have analyzed several well-known anti-mitotic, spindle-targeting compounds, all of which have been reported to induce micronuclei formation and chromosome loss. For each drug, the rate of HAC loss was accurately measured by flow cytometry as a proportion of non-fluorescent cells in the cell population which was verified by FISH analysis. Based on our estimates, despite their similar cytotoxicity, the analyzed drugs affect the rates of HAC mis-segregation during mitotic divisions differently. The highest rate of HAC mis-segregation was observed for the microtubule-stabilizing drugs, taxol and peloruside A.Conclusion: Thus, this new and simple assay allows for a quick and efficient screen of hundreds of drugs to identify those affecting chromosome mis-segregation. It also allows ranking of compounds with the same or similar mechanism of action based on their effect on the rate of chromosome loss. The identification of new compounds that increase chromosome mis-segregation rates should expedite the development of new therapeutic strategies to target the CIN phenotype in cancer cells. [ABSTRACT FROM AUTHOR]

Published
2013
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17. Input DNA Ratio Determines Copy Number of The 33 kb Factor IX Gene on De Novo Human Artificial Chromosomes.

Author

Breman, Amy M., Steiner, Camie M., Slee, Roger B., and Grimes, Brenda R.

Subjects
*DNA, *ARTIFICIAL chromosomes, *GENETICS, *GENE therapy, *GENETIC transformation, *THERAPEUTICS, *TRANSGENES
Abstract

Human artificial chromosomes (ACs) are non-integrating vectors that may be useful for gene therapy. They assemble in cultured cells following transfection of human centromeric α -satellite DNA and segregate efficiently alongside the host genome. In the present study, a 33 kilobase (kb) Factor IX (FIX) gene was incorporated into mitotically stable ACs in human HT1080 lung derived cells using co-transfection of a bacterial artificial chromosome (BAC) harboring synthetic α -satellite DNA and a P1 artificial chromosome(PAC) that spans the FIX locus. ACs were detected in ≥90% of chromosome spreads in 8 of 19 lines expanded from drug resistant colonies. FIX transgene copy number on ACs was determined by input DNA transfection ratios. Furthermore, a low level of FIX transcription was detected from ACs with multiple transgenes but not from those incorporating a single transgene, suggesting that reducing transgene number may limit misexpression. Their potential to segregate cross species was measured by transferring ACs into mouse and hamster cell lines using microcell-mediated chromosome transfer. Lines were obtained where ACs segregated efficiently. The stable segregation of ACs in rodent cells suggests that it should be possible to develop animal models to test the capacity of ACs to rescue FIX deficiency.Molecular Therapy (2007); 16 2, 315–323. doi:10.1038/sj.mt.6300361 [ABSTRACT FROM AUTHOR]

Published
2008
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18. Selective inhibition of pancreatic ductal adenocarcinoma cell growth by the mitotic MPS1 kinase inhibitor NMS-P715.

Author

Slee RB, Grimes BR, Bansal R, Gore J, Blackburn C, Brown L, Gasaway R, Jeong J, Victorino J, March KL, Colombo R, Herbert BS, and Korc M

Subjects
Adenocarcinoma genetics, Adenocarcinoma metabolism, Adenocarcinoma pathology, Animals, Apoptosis drug effects, Apoptosis genetics, Blotting, Western, Carcinoma, Pancreatic Ductal genetics, Carcinoma, Pancreatic Ductal metabolism, Carcinoma, Pancreatic Ductal pathology, Cell Cycle Proteins genetics, Cell Cycle Proteins metabolism, Cell Line, Tumor, Dose-Response Relationship, Drug, Gene Expression Regulation, Neoplastic drug effects, Humans, In Situ Hybridization, Fluorescence, Pancreatic Neoplasms genetics, Pancreatic Neoplasms metabolism, Pancreatic Neoplasms pathology, Prognosis, Protein Kinase Inhibitors pharmacology, Protein Serine-Threonine Kinases genetics, Protein Serine-Threonine Kinases metabolism, Protein-Tyrosine Kinases genetics, Protein-Tyrosine Kinases metabolism, Survival Analysis, Time Factors, Transcriptome, Cell Cycle Proteins antagonists & inhibitors, Cell Proliferation drug effects, Protein Serine-Threonine Kinases antagonists & inhibitors, Protein-Tyrosine Kinases antagonists & inhibitors, Pyrazoles pharmacology, Quinazolines pharmacology
Abstract

Most solid tumors, including pancreatic ductal adenocarcinoma (PDAC), exhibit structural and numerical chromosome instability (CIN). Although often implicated as a driver of tumor progression and drug resistance, CIN also reduces cell fitness and poses a vulnerability that can be exploited therapeutically. The spindle assembly checkpoint (SAC) ensures correct chromosome-microtubule attachment, thereby minimizing chromosome segregation errors. Many tumors exhibit upregulation of SAC components such as MPS1, which may help contain CIN within survivable limits. Prior studies showed that MPS1 inhibition with the small molecule NMS-P715 limits tumor growth in xenograft models. In cancer cell lines, NMS-P715 causes cell death associated with impaired SAC function and increased chromosome missegregation. Although normal cells appeared more resistant, effects on stem cells, which are the dose-limiting toxicity of most chemotherapeutics, were not examined. Elevated expression of 70 genes (CIN70), including MPS1, provides a surrogate measure of CIN and predicts poor patient survival in multiple tumor types. Our new findings show that the degree of CIN70 upregulation varies considerably among PDAC tumors, with higher CIN70 gene expression predictive of poor outcome. We identified a 25 gene subset (PDAC CIN25) whose overexpression was most strongly correlated with poor survival and included MPS1. In vitro, growth of human and murine PDAC cells is inhibited by NMS-P715 treatment, whereas adipose-derived human mesenchymal stem cells are relatively resistant and maintain chromosome stability upon exposure to NMS-P715. These studies suggest that NMS-P715 could have a favorable therapeutic index and warrant further investigation of MPS1 inhibition as a new PDAC treatment strategy.

Published
2014
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19. Interphase FISH demonstrates that human adipose stromal cells maintain a high level of genomic stability in long-term culture.

Author

Grimes BR, Steiner CM, Merfeld-Clauss S, Traktuev DO, Smith D, Reese A, Breman AM, Thurston VC, Vance GH, Johnstone BH, Slee RB, and March KL

Subjects
Adult, Blood Vessels cytology, Cell Culture Techniques, Cell Proliferation, Cells, Cultured, Chromosomes, Human genetics, Clone Cells, Female, Humans, Male, Middle Aged, Prenatal Diagnosis, Time Factors, Adipose Tissue cytology, Genomic Instability, In Situ Hybridization, Fluorescence, Interphase, Stromal Cells cytology, Stromal Cells metabolism
Abstract

Human adipose stromal cells (ASCs) reside within the stromal-vascular fraction (SVF) in fat tissue, can be readily isolated, and include stem-like cells that may be useful for therapy. An important consideration for clinical application and functional studies of stem/progenitor cells is their capacity to maintain chromosome stability in culture. In this study, cultured ASC populations and ASC clones were evaluated at intervals for maintenance of chromosome stability. Uncultured SVF (uSVF) cells were included for comparison. G-banded chromosome analysis demonstrated that ASCs are diploid and have a normal karyotype. However since only approximately 20 cells are examined, low levels of chromosome instability would not be detected. To increase detection sensitivity, fluorescence in situ hybridization was employed, to permit chromosome enumeration in larger numbers of interphase cells. Seven cultured ASC populations, two ASC clones and four uSVF samples were examined. Chromosome X and 17 probes identified diploid, tetraploid, and aneuploid interphase cells. Both cultured ASC populations [up to approximately 35 Population Doublings (PDs)] and uSVF cells exhibited a similar level of diploidy (97.8% n = 6,355 and 98.83% n = 1,197, respectively) and numerical abnormalities, suggesting that cultured ASCs are genomically stable and supporting their suitability for transplantation applications. In comparison, cultured primary human chorionic villus cells exhibited marked genomic instability resulting in an 11.6% tetraploidy rate after 8-10 PD. Thus effects of culture on genomic stability may be cell type dependent and should be tested by appropriately scaled interphase fluorescence in situ hybridization analysis in any ex vivo expanded cell population destined for transplantation.

Published
2009
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20. Assembly and characterization of heterochromatin and euchromatin on human artificial chromosomes.

Author

Grimes BR, Babcock J, Rudd MK, Chadwick B, and Willard HF

Subjects
Chromobox Protein Homolog 5, Chromosomal Proteins, Non-Histone genetics, Chromosomal Proteins, Non-Histone metabolism, Chromosomes, Human, Pair 17 genetics, Chromosomes, Human, Pair 17 metabolism, DNA Methylation, DNA Replication genetics, Genetic Variation genetics, Histones genetics, Histones metabolism, Humans, Lysine genetics, Lysine metabolism, Chromosomes, Artificial, Human genetics, Euchromatin genetics, Heterochromatin genetics
Abstract

Background: Human centromere regions are characterized by the presence of alpha-satellite DNA, replication late in S phase and a heterochromatic appearance. Recent models propose that the centromere is organized into conserved chromatin domains in which chromatin containing CenH3 (centromere-specific H3 variant) at the functional centromere (kinetochore) forms within regions of heterochromatin. To address these models, we assayed formation of heterochromatin and euchromatin on de novo human artificial chromosomes containing alpha-satellite DNA. We also examined the relationship between chromatin composition and replication timing of artificial chromosomes., Results: Heterochromatin factors (histone H3 lysine 9 methylation and HP1alpha) were enriched on artificial chromosomes estimated to be larger than 3 Mb in size but depleted on those smaller than 3 Mb. All artificial chromosomes assembled markers of euchromatin (histone H3 lysine 4 methylation), which may partly reflect marker-gene expression. Replication timing studies revealed that the replication timing of artificial chromosomes was heterogeneous. Heterochromatin-depleted artificial chromosomes replicated in early S phase whereas heterochromatin-enriched artificial chromosomes replicated in mid to late S phase., Conclusions: Centromere regions on human artificial chromosomes and host chromosomes have similar amounts of CenH3 but exhibit highly varying degrees of heterochromatin, suggesting that only a small amount of heterochromatin may be required for centromere function. The formation of euchromatin on all artificial chromosomes demonstrates that they can provide a chromosome context suitable for gene expression. The earlier replication of the heterochromatin-depleted artificial chromosomes suggests that replication late in S phase is not a requirement for centromere function.

Published
2004
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21. Alpha-satellite DNA and vector composition influence rates of human artificial chromosome formation.

Author

Grimes BR, Rhoades AA, and Willard HF

Subjects
Cell Line, Centromere physiology, Chromosomes, Artificial, Human physiology, Chromosomes, Human, Pair 21, Chromosomes, Human, Y, Cytogenetic Analysis, Humans, In Situ Hybridization, Fluorescence, Kinetochores physiology, Mitosis, Chromosomes, Artificial, Human genetics, DNA, Satellite genetics, Genetic Vectors
Abstract

Human artificial chromosomes (HACs) have been proposed as a new class of potential gene transfer and gene therapy vector. HACs can be formed when bacterial cloning vectors containing alpha-satellite DNA are transfected into cultured human cells. We have compared the HAC-forming potential of different sequences to identify features critical to the efficiency of the process. Chromosome 17 or 21 alpha-satellite arrays are highly competent HAC-forming substrates in this assay. In contrast, a Y-chromosome-derived alpha-satellite sequence is inefficient, suggesting that centromere specification is at least partly dependent on DNA sequence. The length of the input array is also an important determinant, as reduction of the chromosome-17-based array from 80 kb to 35 kb reduced the frequency of HAC formation. In addition to the alpha-satellite component, vector composition also influenced HAC formation rates, size, and copy number. The data presented here have a significant impact on the design of future HAC vectors that have potential to be developed for therapeutic applications and as tools for investigating human chromosome structure and function., ((c)2002 Elsevier Science (USA).)

Published
2002
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