Your search keyword '"Nona Arneson"' showing total 16 results

1. Mapping genomic and transcriptomic alterations spatially in epithelial cells adjacent to human breast carcinoma

Author

Moustafa Abdalla, Danh Tran-Thanh, Juan Moreno, Vladimir Iakovlev, Ranju Nair, Nisha Kanwar, Mohamed Abdalla, Jennifer P. Y. Lee, Jennifer Yin Yee Kwan, Thomas R. Cawthorn, Keisha Warren, Nona Arneson, Dong-Yu Wang, Natalie S. Fox, Bruce J. Youngson, Naomi A. Miller, Alexandra M. Easson, David McCready, Wey L. Leong, Paul C. Boutros, and Susan J. Done

Subjects

Science

Abstract

Studying the spatial mutational and gene expression alterations in breast cancer could impact our understanding of breast cancer development. Here, the authors analyse a unique dataset of epithelial samples that highlight potential field cancerisation surrounding the primary tumour.

Published

2017

2. Mapping genomic and transcriptomic alterations spatially in epithelial cells adjacent to human breast carcinoma

Author

Thomas R. Cawthorn, Nisha Kanwar, Susan J. Done, Juan C. Moreno, Keisha Warren, Mohamed Abdalla, Naomi Miller, Danh Tran-Thanh, Natalie S. Fox, Vladimir Iakovlev, Jennifer P.Y. Lee, Alexandra M. Easson, Wey L. Leong, Moustafa Abdalla, Paul C. Boutros, Nona Arneson, Ranju Nair, Bruce Youngson, Jennifer Y. Y. Kwan, David R. McCready, and Dong-Yu Wang

Subjects

0301 basic medicine, Messenger, General Physics and Astronomy, Cell Cycle Proteins, Transcriptome, 0302 clinical medicine, Ductal, 2.1 Biological and endogenous factors, Breast, Aetiology, lcsh:Science, skin and connective tissue diseases, Oligonucleotide Array Sequence Analysis, Cancer, Genetics, Comparative Genomic Hybridization, Multidisciplinary, Tissue microarray, Genome, Carcinoma, Ductal, Breast, RNA-Binding Proteins, Genomics, 030220 oncology & carcinogenesis, MCF-7 Cells, Female, Human, Biotechnology, Science, Breast Neoplasms, Biology, Article, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Breast cancer, Clinical Research, Breast Cancer, medicine, Carcinoma, Humans, RNA, Messenger, Genome, Human, Gene Expression Profiling, Human Genome, Epithelial Cells, General Chemistry, medicine.disease, Human genetics, Gene expression profiling, 030104 developmental biology, Mutation, Cancer research, RNA, lcsh:Q, Field cancerization, Neoplasm Grading, Comparative genomic hybridization

Abstract

Almost all genomic studies of breast cancer have focused on well-established tumours because it is technically challenging to study the earliest mutational events occurring in human breast epithelial cells. To address this we created a unique dataset of epithelial samples ductoscopically obtained from ducts leading to breast carcinomas and matched samples from ducts on the opposite side of the nipple. Here, we demonstrate that perturbations in mRNA abundance, with increasing proximity to tumour, cannot be explained by copy number aberrations. Rather, we find a possibility of field cancerization surrounding the primary tumour by constructing a classifier that evaluates where epithelial samples were obtained relative to a tumour (cross-validated micro-averaged AUC = 0.74). We implement a spectral co-clustering algorithm to define biclusters. Relating to over-represented bicluster pathways, we further validate two genes with tissue microarrays and in vitro experiments. We highlight evidence suggesting that bicluster perturbation occurs early in tumour development., Studying the spatial mutational and gene expression alterations in breast cancer could impact our understanding of breast cancer development. Here, the authors analyse a unique dataset of epithelial samples that highlight potential field cancerisation surrounding the primary tumour.

Published

2017

3. Genomic Differences Between Pure Ductal Carcinoma In Situ of the Breast and that Associated with Invasive Disease: a Calibrated aCGH Study

Author

Vladimir Iakovlev, Nona Arneson, Gaiane Iakovleva, Keisha Warren, Melania Pintilie, Chunjie Wang, Susan J. Done, Vietty Wong, and Stephanie Leung

Subjects

Adult, In situ, Cancer Research, Pathology, medicine.medical_specialty, Clone (cell biology), Breast Neoplasms, Biology, medicine, Humans, skin and connective tissue diseases, neoplasms, Lymph node, Aged, Oligonucleotide Array Sequence Analysis, Aged, 80 and over, Reverse Transcriptase Polymerase Chain Reaction, Carcinoma, Ductal, Breast, Cancer, Middle Aged, Ductal carcinoma, medicine.disease, body regions, Carcinoma, Intraductal, Noninfiltrating, medicine.anatomical_structure, Lymphatic system, Oncology, Female, Lymph, Chromosomes, Human, Pair 17, Comparative genomic hybridization

Abstract

Purpose: In the quest for new targets, genomes of ductal carcinoma in situ (DCIS) and infiltrating duct carcinoma (IDC) have been compared previously; however, genomic alterations associated with cancer progression were difficult to identify. We hypothesized that significant events can be detected by comparing lesions with a broader range of behavior: from pure DCIS to IDC associated with lymph node metastasis. Experimental Design: Array comparative genomic hybridization, calibrated by self-self hybridization tests, was used to study 6 cases of pure DCIS and 17 cases of DCIS paired with IDC where 8 tumors had spread to the local lymph nodes. Results: Pure DCIS exhibited a marginally higher degree of genomic complexity than DCIS and IDC components of invasive tumors. The latter two showed similarity between tumors and between components of the same tumor with several regions detected preferentially compared with pure DCIS. IDC associated with lymph node metastases showed similarity of genomic profiles as a group. Gain on 17q22-24.2 was associated with higher histologic grade, large IDC size, lymphatic/vascular invasion, and lymph node metastasis (P < 0.05). Conclusions: Our findings suggest that DCIS and IDC are associated with specific genomic events. DCIS associated with IDC is genomically similar to the invasive component and therefore may represent either a clone with high invasive potential or invasive cancer spreading through the ducts. Specifically, gain on 17q22-24.2 is a candidate region for further testing as a predictor of invasion when detected in DCIS and predictor of nodal metastasis when detected in DCIS or IDC.

Published

2008

4. Genomic Alterations in Sporadic Synchronous Primary Breast Cancer Using Array and Metaphase Comparative Genomic Hybridization

Author

Arezou A. Ghazani, Nona Arneson, Melania Pintilie, Susan J. Done, Keisha Warren, Jeremy A. Squire, and Jane Bayani

Subjects

Genetics, Cancer Research, array CGH (aCGH), In situ hybridization, Biology, medicine.disease, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, Genome, lcsh:RC254-282, microdissection, Breast cancer, metaphase CGH (mCGH), comparative genomic hybridization (CGH), medicine, Cancer research, Carcinoma, Human genome, Synchronous breast cancer, Metaphase, Microdissection, Comparative genomic hybridization

Abstract

Synchronous primary breast cancer describes the occurrence of multiple tumors affecting one or both breasts at initial diagnosis. This provides a unique opportunity to identify tissue-specific genomic markers that characterize each tumor while controlling for the individual genetic background of a patient. The aim of this study was to examine the genomic alterations and degree of similarity between synchronous cancers. Using metaphase comparative genomic hybridization and array comparative genomic hybridization (aCGH), the genomic alterations of 23 synchronous breast cancers from 10 patients were examined at both chromosomal and gene levels. Synchronous breast cancers, when compared to their matched counterparts, were found to have a common core set of genetic alterations, with additional unique changes present in each. They also frequently exhibited features distinct from the more usual solitary primary breast cancers. The most frequent genomic alterations included chromosomal gains of 1q, 3p, 4q, and 8q, and losses of 11q, 12q, 16q, and 17p. aCGH identified copy number amplification in regions that are present in all 23 tumor samples, including 1p31.3–1p32.3 harboring JAK1. Our findings suggest that synchronous primary breast cancers represent a unique type of breast cancer and, at least in some instances, one tumor may give rise to the other.

Published

2007

5. Comparison of HER2/neuStatus Assessed by Quantitative Polymerase Chain Reaction and Immunohistochemistry

Author

Frances P. O'Malley, Nona Arneson, Eleanor Latta, Suzanna Tjan, Tanya Zadro, Robert Parkes, Irene L. Andrulis, Rosemary E. Mueller, and Martin E. Blackstein

Subjects

Canada, Pathology, medicine.medical_specialty, Receptor, ErbB-2, Biopsy, Concordance, Breast Neoplasms, Biology, Antibodies, Monoclonal, Humanized, HER2/Neu Status, Polymerase Chain Reaction, Sensitivity and Specificity, HercepTest, law.invention, Predictive Value of Tests, law, Gene duplication, Carcinoma, medicine, Humans, Neoplasm Invasiveness, Prospective Studies, Polymerase chain reaction, Immunization, Passive, Antibodies, Monoclonal, General Medicine, Trastuzumab, medicine.disease, Immunohistochemistry, Molecular biology, Real-time polymerase chain reaction, Female, Reagent Kits, Diagnostic

Abstract

We prospectively evaluated a series of 254 breast cancers by quantitative polymerase chain reaction (PCR) and immunohistochemistry using 3 antibodies: HercepTest, CB11, and TAB250. DNA was extracted from a 10-micron tumor section for PCR, and 4-micron serial sections were taken from the same block for immunohistochemistry. The immunohistochemical results were scored using a semiquantitative immunohistochemical system. A positive tumor by immunohistochemistry had a score of 5 or more. The manufacturer's recommended scoring system was used for the HercepTest. Tumors were positive for gene amplification if the ratio of the HER2/neu gene to control gene after normalization was 2 or more. Of 254 cases, 61 showed gene amplification. For immunohistochemistry, 23% of tumors were positive with CB11, 27% with TAB250, and 37% with the HercepTest. Results for each antibody were compared with PCR results. The overall concordance for the HercepTest was 82%, which was significantly lower than that for CB11 (88%) or TAB250 (87%). The specificity for the HercepTest was 80% compared with 90% for TAB250 and 93% for CB11, while the positive predictive value for the HercepTest was 57% compared with 71% and 76% for TAB250 and CB11, respectively.

Published

2001

6. Comparison of whole genome amplification methods for analysis of DNA extracted from microdissected early breast lesions in formalin-fixed paraffin-embedded tissue

Author

Susan J. Done, Arezou A. Ghazani, Juan A. Moreno, Vladimir Iakovlev, Keisha Warren, Igor Jurisica, Nona Arneson, and David McCready

Subjects

Whole Genome Amplification, Pathology, medicine.medical_specialty, Formalin fixed paraffin embedded, Article Subject, Cancer, Degenerate oligonucleotide, Biology, medicine.disease, Molecular biology, chemistry.chemical_compound, Real-time polymerase chain reaction, Breast cancer, chemistry, medicine, DNA, Comparative genomic hybridization, Research Article

Abstract

To understand cancer progression, it is desirable to study the earliest stages of its development, which are often microscopic lesions. Array comparative genomic hybridization (aCGH) is a valuable high-throughput molecular approach for discovering DNA copy number changes; however, it requires a relatively large amount of DNA, which is difficult to obtain from microdissected lesions. Whole genome amplification (WGA) methods were developed to increase DNA quantity; however their reproducibility, fidelity, and suitability for formalin-fixed paraffin-embedded (FFPE) samples are questioned. Using aCGH analysis, we compared two widely used approaches for WGA: single cell comparative genomic hybridization protocol (SCOMP) and degenerate oligonucleotide primed PCR (DOP-PCR). Cancer cell line and microdissected FFPE breast cancer DNA samples were amplified by the two WGA methods and subjected to aCGH. The genomic profiles of amplified DNA were compared with those of non-amplified controls by four analytic methods and validated by quantitative PCR (Q-PCR). We found that SCOMP-amplified samples had close similarity to non-amplified controls with concordance rates close to those of reference tests, while DOP-amplified samples had a statistically significant amount of changes. SCOMP is able to amplify small amounts of DNA extracted from FFPE samples and provides quality of aCGH data similar to non-amplified samples.

Published

2011

7. Whole-Genome Amplification by Improved Primer Extension Preamplification PCR (I-PEP-PCR)

Author

Nona Arneson, Simon Hughes, Susan J. Done, and Richard S. Houlston

Subjects

Exonuclease, Whole Genome Amplification, biology, DNA polymerase, Chemistry, Multiple displacement amplification, Molecular biology, General Biochemistry, Genetics and Molecular Biology, Primer extension, chemistry.chemical_compound, biology.protein, Proofreading, Polymerase, DNA

Abstract

INTRODUCTIONPCR-based whole-genome amplification (WGA) has the goal of generating microgram quantities of genome-representative DNA from picogram or nanogram amounts of starting material. This amplification should introduce little, or ideally no, representational bias. In contrast to other techniques for WGA, PCR-based methods are generally less affected by DNA quality and are more applicable to DNA extracted from various sources (fixed and fresh tissues). Primer extension preamplification PCR (PEP-PCR), in contrast to degenerate oligonucleotide primed PCR (DOP-PCR), uses totally degenerate 15-mer PCR primers. An additional difference is that in PEP-PCR, the number of potential priming sites is orders of magnitude larger. The effectiveness of PEP-PCR has been increased by several alterations. The improved PEP (I-PEP) PCR approach, described in this protocol, uses a DNA polymerase cocktail that includes Taq DNA polymerase (to carry out the primer extension as in a traditional PCR) and a proofreading DNA polymerase (to provide 3′-to-5′-exonuclease activity, excising misincorporated nucleotides that slow the progression of Taq DNA polymerase). The result is far more efficient WGA, with increased fidelity due to the removal of the misincorporated nucleotides. Similar to DOP-PCR, PEP-PCR generates a smear of DNA fragments that are visible on an agarose gel.

Published

2011

8. Whole-Genome Amplification by Degenerate Oligonucleotide Primed PCR (DOP-PCR)

Author

Simon Hughes, Nona Arneson, Richard S. Houlston, and Susan J. Done

Subjects

Whole Genome Amplification, XhoI, biology, Chemistry, Multiple displacement amplification, Random hexamer, Genome, Molecular biology, General Biochemistry, Genetics and Molecular Biology, chemistry.chemical_compound, Restriction site, biology.protein, Human genome, DNA

Abstract

INTRODUCTIONPCR-based whole-genome amplification (WGA) has the goal of generating microgram quantities of genome-representative DNA from picogram or nanogram amounts of starting material. This amplification should introduce little, or ideally no, representational bias. Unlike other techniques for WGA, PCR-based methods are generally less affected by DNA quality and are more applicable to DNA extracted from various sources (fixed and fresh tissues). The degenerate-oligonucleotide-primed PCR (DOP-PCR) method described here allows complete genome coverage in a single reaction. In contrast to the pairs of target-specific primer sequences used in traditional PCR, only a single primer, which has defined sequences at its 5′-end (containing an XhoI restriction site) and 3′-end and a random hexamer sequence between them, is used here. DOP-PCR comprises two different cycling stages. In stage 1 (low stringency), low-temperature annealing and extension in the first five to eight cycles occurs at many binding sites in the genome. The 3′-end of the primer binds at sites in the genome complementary to the 6-bp well-defined sequence at the 3′-end of the primer (~106 sites in the human genome). The adjacent random hexamer sequence (displaying all possible combinations of the nucleotides A, G, C, and T) can then anneal and tags these sequences with the DOP primer. In stage 2 (high stringency; >25 cycles), the PCR annealing temperature is raised, which increases priming specificity during amplification of the tagged sequence. DOP-PCR generates a smear of DNA fragments (200-1000 bp) that are visible on an agarose gel.

Published

2011

9. Amplification of the prolactin receptor gene in mammary lobular neoplasia

Author

Anita Bane, Melania Pintilie, Susan J. Done, Ardit Deliallisi, Danh Tran-Thanh, Keisha Warren, and Nona Arneson

Subjects

Adult, Cancer Research, Pathology, medicine.medical_specialty, Receptors, Prolactin, Mammary gland, Lobular carcinoma, Copy number analysis, Breast Neoplasms, Biology, Breast cancer, medicine, STAT5 Transcription Factor, Humans, skin and connective tissue diseases, neoplasms, Aged, Aged, 80 and over, Comparative Genomic Hybridization, Prolactin receptor, Carcinoma in situ, Tumor Suppressor Proteins, Gene Amplification, Middle Aged, medicine.disease, Cadherins, body regions, Carcinoma, Lobular, medicine.anatomical_structure, Oncology, Cancer research, Chromosomes, Human, Pair 5, Female, Breast disease, Lobular Neoplasia, Genome-Wide Association Study

Abstract

The identification of lobular carcinoma in situ (LCIS) in a patient's specimen confers an appreciable increased risk of development of future invasive mammary carcinoma. However, the study of LCIS presents a challenge as it is usually only recognized in fixed specimens. Recent advances in high throughput genomics have made possible comprehensive copy number analysis of lesions such as this. Using array comparative genomic hybridization (aCGH), we characterized eight cases of lobular carcinoma (four invasive and four non-invasive) from microdissected samples of archival specimens and validated our results by quantitative real-time PCR (qRT-PCR). Immunohistochemistry (IHC) was performed on an independent set of 80 in situ ductal (DCIS) and lobular breast lesions to confirm our results. Amplification of the prolactin receptor gene (PRLr) was identified in 4/4 cases of LCIS by aCGH. We confirmed this amplification by qRT-PCR and demonstrated PRLr expression in 29/40 (73%) cases of lobular neoplasia by IHC. Amplification of PRLr was neither detected in 10 cases of DCIS nor in 5 areas of normal breast tissue by qRT-PCR and only 14/40 (35%) cases of DCIS showed PRLr expression by IHC (P = 0.0008). Our study suggests the prolactin receptor gene is a molecular target that may be important in the pathogenesis and progression of lobular neoplasia. Investigation of the status of this gene in cases of DCIS has indicated that it may not be as important in the progression of this type of breast cancer, supporting the view that lobular and ductal carcinomas may evolve along separate pathways.

Published

2010

10. Genomic alterations in primary breast cancers compared with their sentinel and more distal lymph node metastases: an aCGH study

Author

Gaiane Iakovleva, Chunjie Wang, Naomi Miller, Bruce Youngson, Susan J. Done, Stephanie Leung, Vladimir Iakovlev, Melania Pintilie, David R. McCready, Keisha Warren, Nona Arneson, and Vietty Wong

Subjects

Adult, Cancer Research, Pathology, medicine.medical_specialty, Breast Neoplasms, Biology, Polymerase Chain Reaction, Metastasis, Immunoenzyme Techniques, Breast cancer, Genetics, medicine, Humans, skin and connective tissue diseases, neoplasms, Lymph node, Aged, Neoplasm Staging, Oligonucleotide Array Sequence Analysis, Comparative Genomic Hybridization, Tumor size, Genome, Human, Sentinel Lymph Node Biopsy, Nodal metastasis, Carcinoma, Ductal, Breast, Middle Aged, medicine.disease, Prognosis, medicine.anatomical_structure, Lymphatic Metastasis, Female, Lymph, Lymph Nodes, NODAL, Comparative genomic hybridization, Chromosomes, Human, Pair 17

Abstract

Metastatic potential of breast cancer may be associated with specific genomic alterations and the earliest metastases are likely to be found in the sentinel lymph nodes (SLN). Using array comparative genomic hybridization (aCGH), we compared the genomes of primary breast invasive duct carcinomas (IDCs), their sentinel and more distal lymph node metastases, and IDCs without nodal metastasis. Thirty-three samples from 22 patients with IDC were subjected to aCGH: 8 IDC samples from patients without lymph node metastasis, 11 IDCs associated with SLN metastases out of which 7 had paired samples of metastases, and 14 samples of lymph node metastases out of which 8 were sentinel-distal pairs from 4 patients. aCGH data were analyzed by correlation of genomic profiles, cluster analysis, segmentation, and peak identification. Quantitative real-time PCR was used for data validation. We observed high genomic similarity between primary tumors and their nodal metastases as well as between metastases to the sentinel and distal lymph nodes. Several recurrent alterations were detected preferentially in IDC associated with SLN metastases compared to IDCs without metastasis. Amplification within the 17q24.1-24.2(59.96–62.76 Mb) region was associated with presence of sentinel or distal lymph node metastases; larger tumor size and higher histological grade. In our samples, there were genomic events associated with metastatic progression, which could be detected in both primary tumors and LN metastases. Gain on 17q24.1-24.2 is a candidate region for further testing as a predictor of nodal metastasis. © 2009 Wiley-Liss, Inc.

Published

2009

11. Limited tissue fixation times and whole genomic amplification do not impact array CGH profiles

Author

Arezou A. Ghazani, Nona Arneson, Susan J. Done, and Keisha Warren

Subjects

Genetic Markers, Time Factors, Microarray, Genomics, Breast Neoplasms, Biology, Genome, Sensitivity and Specificity, Pathology and Forensic Medicine, Cell Line, Tumor, Humans, Oligonucleotide Array Sequence Analysis, Retrospective Studies, Whole Genome Amplification, Paraffin Embedding, Gene Expression Profiling, Chromosome Mapping, Nucleic Acid Hybridization, General Medicine, Nucleic acid amplification technique, Molecular biology, Gene expression profiling, Genetic marker, Case-Control Studies, Original Article, Female, Nucleic Acid Amplification Techniques, Comparative genomic hybridization

Abstract

Array comparative genomic hybridisation (CGH) is a powerful method for the genetic analysis of lesional and normal tissues to identify genomic imbalances associated with malignancies. However, the use of this technique with DNA extracted from archival formalin fixed, paraffin embedded (FFPE) tissue specimens, the most widely available resource for retrospective studies, is subject to quantitative and qualitative limitations. In this report, the suitability and integrity of the DNA extracted from FFPE MCF7 breast cancer cells fixed for different periods of time for array CGH applications were examined.Using our established cDNA microarray protocol in conjunction with whole genome amplification methods, the genetic profiles of freshly harvested MCF7 cells and their matched FFPE counterparts were analysed. Congruent profiles between FFPE MCF7 cells and their fresh counterpart and between amplified and non-amplified FFPE MCF7 cells were observed. Our results demonstrate that formalin fixation of20 hours has no significant adverse effect on the integrity of DNA for array CGH studies.Our findings attest to the fidelity of our array CGH methods to effectively examine material recovered from FFPE tissue specimens for microarray applications. This in turn has great potential to identify novel diagnostic and prognostic markers for human disease.

Published

2006

12. The use of whole genome amplification in the study of human disease

Author

Nona Arneson, Susan J. Done, Jeremy A. Squire, and Simon Hughes

Subjects

Whole Genome Amplification, Genetics, Genome, Human, Linear amplification, Biophysics, DNA-Directed DNA Polymerase, Biology, Genome, Polymerase Chain Reaction, law.invention, genomic DNA, chemistry.chemical_compound, Human disease, chemistry, law, Humans, Molecular Biology, Nucleic Acid Amplification Techniques, Polymerase chain reaction, DNA

Abstract

The availability of large amounts of genomic DNA is of critical importance for many of the molecular biology assays used in the analysis of human disease. However, since the amount of patient tissue available is often limited and as particular foci of interest may consist of only a few hundred cells, the yield of DNA is often insufficient for extensive analysis. To address this problem, several whole genome amplification (WGA) methodologies have been developed. Initial WGA approaches were based on the polymerase chain reaction (PCR). However, recent reports have described the use of non-PCR-based linear amplification protocols for WGA. Using these methods, it is possible to generate microgram quantities of DNA starting with as little as 1mg of genomic DNA. This review will provide an overview of WGA approaches and summarize some of the uses for amplified DNA in various high-throughput genetic applications.

Published

2004

13. Whole-Genome Amplification by Single-Cell Comparative Genomic Hybridization PCR (SCOMP)

Author

Simon Hughes, Nona Arneson, Susan J. Done, and Richard S. Houlston

Subjects

Whole Genome Amplification, genomic DNA, Restriction enzyme, chemistry.chemical_compound, Chemistry, Agarose gel electrophoresis, Multiple displacement amplification, Genome, Molecular biology, General Biochemistry, Genetics and Molecular Biology, DNA, Comparative genomic hybridization

Abstract

INTRODUCTIONPCR-based whole-genome amplification (WGA) has the goal of generating microgram quantities of genome-representative DNA from picogram or nanogram amounts of starting material. This amplification should introduce little, or ideally no, representational bias. In contrast to other techniques for WGA, PCR-based methods are generally less affected by DNA quality and are more applicable to DNA extracted from various sources (fixed and fresh tissues). Ligation-mediated PCR techniques involve ligating an adaptor sequence onto a “representation” of DNA molecules, generated following enzymatic digestion, random shearing, or chemical cleavage. Single-cell comparative genomic hybridization (SCOMP), described in this protocol, is a form of ligation-mediated PCR that was specifically designed for WGA of extremely limited sources of genomic DNA. The reaction volume is purposely kept to a minimum, and all buffers are optimized to eliminate the need to purify the reaction between steps. In addition, the entire reaction is performed in a single tube. This avoids initial template loss and reduces the risk of PCR contamination. SCOMP begins by converting the genome to a high-complexity representation with a fragment size of

Published

2008

14. GenomePlex Whole-Genome Amplification

Author

Richard S. Houlston, Simon Hughes, Susan J. Done, and Nona Arneson

Subjects

genomic DNA, chemistry.chemical_compound, chemistry, Biochemistry, GenomePlex, MALBAC, Multiple displacement amplification, Genome, GenomePlex Whole Genome Amplification, General Biochemistry, Genetics and Molecular Biology, DNA, In vitro

Abstract

INTRODUCTIONPCR-based whole-genome amplification (WGA) has the goal of generating microgram quantities of genome-representative DNA from picogram or nanogram amounts of starting material. This amplification should introduce little, or ideally no, representational bias. In contrast to other techniques for WGA, PCR-based methods are generally less affected by DNA quality and are more applicable to DNA extracted from various sources (fixed and fresh tissues). GenomePlex WGA, described in this protocol, is a proprietary amplification technology based on nonenzymatic random fragmentation of genomic DNA. The protocol involves conversion of the genome into an in vitro molecular library of DNA fragments, followed by incubation at various temperatures to add adaptor sequences with specific PCR priming sites to both ends of every fragment. The fragment library can then be amplified several 1000-fold to generate milligram quantities of DNA starting with as little as 10-100 ng.

Published

2008

15. Whole-Genome Amplification by Adaptor-Ligation PCR of Randomly Sheared Genomic DNA (PRSG)

Author

Richard S. Houlston, Nona Arneson, Simon Hughes, and Susan J. Done

Subjects

Whole Genome Amplification, chemistry.chemical_compound, genomic DNA, chemistry, Multiple displacement amplification, Genomic library, Ligation, Genome, Molecular biology, General Biochemistry, Genetics and Molecular Biology, DNA, Chemical Cleavage

Abstract

INTRODUCTIONPCR-based whole-genome amplification (WGA) has the goal of generating microgram quantities of genome-representative DNA from picogram or nanogram amounts of starting material. This amplification should introduce little, or ideally no, representational bias. In contrast to other techniques for WGA, PCR-based methods are generally less affected by DNA quality and are more applicable to DNA extracted from various sources (fixed and fresh tissues). Ligation-mediated PCR techniques involve ligating an adaptor sequence onto a “representation” of DNA molecules, generated following enzymatic digestion, random shearing, or chemical cleavage. Adaptor-ligation PCR of randomly sheared genomic DNA (PRSG), described here, is based on ligation-mediated PCR and was designed to improve genome coverage. Rather than using enzymatically generated fragments, this method uses randomly fragmented DNA as the template. The process involves three steps: (1) the hydrodynamic shearing of genomic DNA to a 0.5-2-kb size range, (2) end filling and adaptor ligation, and (3) high-stringency PCR for faithful replication of the resulting fragments.

Published

2008

16. Quantitative detection of circulating epithelial cells by Q-RT-PCR.

Author

Jonathan Vecchiarelli and Nona Arneson

Subjects

MEDICAL research, BREAST cancer, EPITHELIAL cells, THERAPEUTICS

Abstract

Abstract Introduction    It has been shown that the quantity of circulating tumor cells (CTCs) in breast cancer patients is an independent predictor of survival and treatment response. Real time quantitative reverse transcriptase PCR (Q-RT-PCR) is a sensitive technique for detection of CTCs. Our aim was to investigate whether the technique can be used also to quantitate these CTCs. Methods    We tested cytokeratin 19 (CK19), maspin, mammaglobin, GAPDH and RPL19 genes for their level of expression and linearity of amplification in serial dilutions of RNA extracted from the MDA-MB-231, UACC-812, T47D and HS578T breast cancer cell lines. To simulate CTCs, serial dilutions of cultured T47D and HS578T cells were added to peripheral blood from healthy volunteers. The samples were subjected to enrichment, RNA extraction and Q-RT-PCR. Results   CK19 was reliably expressed in all four cell lines with a linear relationship between the quantity of added cells and the amount of CK19 RNA. The lower limit of reliable detection was 5 cells per sample, which corresponds to a concentration of 0.7 cell/ml in 7.5 ml of blood or would translate to a lower CTC concentration in a larger volume of blood. Conclusion   This technique may prove useful for high throughput comparative quantification of CTCs in individual patients during treatment and subsequent follow up for research and clinical management purposes. [ABSTRACT FROM AUTHOR]

Published

2008