ABSTRACT
Cell viability, an essential measurement for cell therapy products, lacks traceability. One of the most common cell viability tests is trypan blue dye exclusion where blue-stained cells are counted via brightfield imaging. Typically, live and dead cells are classified based on their pixel intensities which may vary arbitrarily making it difficult to compare results. Herein, a traceable absorbance microscopy method to determine the intracellular uptake of trypan blue is demonstrated. The intensity pixels of the brightfield images are converted to absorbance images which are used to calculate moles of trypan blue per cell. Trypan blue cell viability measurements, where trypan blue content in each cell is quantified, enable traceable live-dead classifications. To implement the absorbance microscopy method, we developed an open-source AbsorbanceQ application that generates quantitative absorbance images. The validation of absorbance microscopy is demonstrated using neutral density filters. Results from four different microscopes demonstrate a mean absolute deviation of 3% from the expected optical density values. When assessing trypan blue-stained Jurkat cells, the difference in intracellular uptake of trypan blue in heat-shock-killed cells using two different microscopes is 3.8%. Cells killed with formaldehyde take up ~50% less trypan blue as compared to the heat-shock-killed cells, suggesting that the killing mechanism affects trypan blue uptake. In a test mixture of approximately 50% live and 50% dead cells, 53% of cells were identified as dead (±6% standard deviation). Finally, to mimic batches of low-viability cells that may be encountered during a cell manufacturing process, viability was assessed for cells that were 1) overgrown in the cell culture incubator for five days or 2) incubated in DPBS at room temperature for five days. Instead of making live-dead classifications using arbitrary intensity values, absorbance imaging yields traceable units of moles that can be compared, which is useful for assuring quality for biomanufacturing processes.
Subject(s)
Cell Culture Techniques/methods , Jurkat Cells/cytology , Trypan Blue/chemistry , Cell Count , Cell Survival/drug effects , Formaldehyde/adverse effects , Humans , Jurkat Cells/chemistry , MicroscopyABSTRACT
Azaspiracid-34 (AZA34) is a recently described structurally unique member of the azaspiracid class of marine neurotoxins. Its novel structure, tentatively assigned on the basis of MS and 1H NMR spectroscopy, is accompanied by a 5.5-fold higher level of toxicity against Jurkat T lymphocytes than AZA1. To completely assign the structure of AZA34 and provide material for in-depth biological evaluation and detection, synthetic access to AZA34 was targeted. This began with the convergent and stereoselective assembly of the C1-C19 domain of AZA34 designed to dovetail with the recent total synthesis approach to AZA3.
Subject(s)
Jurkat Cells/cytology , Marine Toxins/toxicity , Neurotoxins/toxicity , Spiro Compounds/chemical synthesis , Humans , Jurkat Cells/chemistry , Magnetic Resonance Spectroscopy , Marine Toxins/chemical synthesis , Marine Toxins/chemistry , Molecular Structure , Spiro Compounds/chemistryABSTRACT
We apply hierarchical clustering (HC) of DNA k-mer counts on multiple Fastq files. The tree structures produced by HC may reflect experimental groups and thereby indicate experimental effects, but clustering of preparation groups indicates the presence of batch effects. Hence, HC of DNA k-mer counts may serve as a diagnostic device. In order to provide a simple applicable tool we implemented sequential analysis of Fastq reads with low memory usage in an R package (seqTools) available on Bioconductor. The approach is validated by analysis of Fastq file batches containing RNAseq data. Analysis of three Fastq batches downloaded from ArrayExpress indicated experimental effects. Analysis of RNAseq data from two cell types (dermal fibroblasts and Jurkat cells) sequenced in our facility indicate presence of batch effects. The observed batch effects were also present in reads mapped to the human genome and also in reads filtered for high quality (Phred > 30). We propose, that hierarchical clustering of DNA k-mer counts provides an unspecific diagnostic tool for RNAseq experiments. Further exploration is required once samples are identified as outliers in HC derived trees.
Subject(s)
Sequence Analysis, DNA/methods , Sequence Analysis, RNA/methods , Software , Data Accuracy , Databases, Genetic/standards , Fibroblasts/chemistry , Humans , Jurkat Cells/chemistry , Sequence Analysis, DNA/standards , Sequence Analysis, RNA/standardsABSTRACT
Antiproliferative effects of 15 sulfides were investigated in human leukemia Jurkat cells. Treatment with 5-50 µM of nine monosulfides and two linear disulfides did not induce DNA fragmentation. Whereas, furan-containing sulfur flavors including methyl 2-methyl-3-furyl disulfide (MMFDS), bis (2-methyl-3-furyl) disulfide (BMFDS), methyl furfuryl disulfide (MFDS) and difurfuryl disulfide (DFDS) induced DNA fragmentation to a varying extent in Jurkat cells. The cell viability-reduction effect of these sulfur flavors was in the following order: DFDS>BMFDS>MMFDS>>MFDS based on the IC50 values. MMFDS and BMFDS, but not DFDS, significantly increased the intracellular ROS level by 1.90- and 3.02-fold, respectively. Addition of N-acetylcysteine (NAC) or glutathione (GSH) partially suppressed induction of DNA fragmentation, apoptosis and caspase-3 activation by MMFDS and BMFDS. These results suggest that the furan-containing disulfides have a strong antiproliferative effect, and the oxidative stress and subsequent caspase-3 activation are involved in antiproliferative effect induced by MMFDS and BMFDS in Jurkat cells.
Subject(s)
Furans/pharmacology , Jurkat Cells/chemistry , Sulfur/pharmacology , Apoptosis , Cell Survival , Humans , Leukemia , Oxidative StressABSTRACT
The study of the regulatory roles in small RNAs can be accelerated by techniques that permit simple, low-cost, and rapid extraction of small RNAs from a small number of cells. In order to ensure highly specific and sensitive detection, the extracted RNAs should be free of the background nucleic acids and present stably in a small volume. To meet these criteria, we designed a multi-well/multi-channel (M&M) chip to carry out automatic and selective isolation of small RNAs via solid-phase extraction (SPE), followed by reverse-transcription (RT) to convert them to the more stable cDNAs in a final volume of 2 µL. Droplets containing buffers for RNA binding, washing, and elution were trapped in microwells, which were connected by one channel, and suspended in mineral oil. The silica magnetic particles (SMPs) for SPE were moved along the channel from well to well, i.e. in between droplets, by a fixed magnet and a translation stage, allowing the nucleic acid fragments to bind to the SMPs, be washed, and then be eluted for RT reaction within 15 minutes. RNAs shorter than 63 nt were selectively enriched from cell lysates, with recovery comparable to that of a commercial kit. Physical separation of the droplets on our M&M chip allowed the usage of multiple channels for parallel processing of multiple samples. It also permitted smooth integration with on-chip RT-PCR, which simultaneously detected the target microRNA, mir-191, expressed in fewer than 10 cancer cells. Our results have demonstrated that the M&M chip device is a valuable and cost-saving platform for studying small RNA expression patterns in a limited number of cells with reasonable sample throughput.
Subject(s)
MicroRNAs/isolation & purification , Microfluidic Analytical Techniques/instrumentation , RNA/isolation & purification , HEK293 Cells/chemistry , Humans , Jurkat Cells/chemistry , RNA/analysis , Reverse Transcriptase Polymerase Chain Reaction , Solid Phase Extraction/methodsABSTRACT
Stable cyclic adenosine 5'-diphosphate ribose (cADPR) analogues are chemical biology tools that can probe the Ca(2+) release mechanism and structure-activity relationships of this emerging potent second messenger. However, analogues with an intact "northern" ribose have been inaccessible due to the difficulty of generating the sensitive N1-ribosyl link. We report the first total synthesis of the membrane permeant, hydrolytically stable, cADPR receptor agonist 8-Br-N1-cIDPR via regio- and stereoselective N1-ribosylation of protected 8-bromoinosine.
Subject(s)
Calcium/chemistry , Calcium/metabolism , Cyclic ADP-Ribose/analogs & derivatives , Cyclic ADP-Ribose/chemical synthesis , Jurkat Cells/chemistry , Cyclic ADP-Ribose/metabolism , Humans , Stereoisomerism , Structure-Activity RelationshipABSTRACT
FCM is a generally accepted tool to analyze apoptosis. Unfortunately, the cell preparation of all commercial kits available includes cell washing known to cause cell loss which is most likely to affect apoptotic cells in particular. To address this, we developed a seven-color single-platform no-wash analysis technique and compared the results with those from an analogous procedure including cell washing. A five-color mAb cocktail was employed to address target cells by surface labeling, Yo-PRO-1® and DAPI were used to discriminate apoptotic and necrotic from viable cells. Cells were quantified on the basis of internal-standard fluorescent beads. Jurkat cells ACC 282 treated with camptothecin were employed to establish the staining procedure, which was then applied to blood cells collected by extracorporeal apheresis and treated with UV irradiation. Data evaluation showed that although each method by itself was highly reproducible (R(2) = 0.973), the numbers of apoptotic cells detected with the no-wash procedure were significantly higher than those obtained after cell washing (P = 6.6 E(-5), Wilcoxon Test). In addition, the observed differences increased with higher cell numbers (Bland and Altmann). We conclude that the described test is a feasible and reliable tool for apoptosis measurement and it provides results that are definitely closer to the truth than those obtained from kits that require cell washing.
Subject(s)
Apoptosis/physiology , Flow Cytometry/methods , Leukemia, T-Cell/pathology , Antibodies, Monoclonal/chemistry , Antineoplastic Agents, Phytogenic/toxicity , Camptothecin/toxicity , Cell Count/methods , Cell Separation , Flow Cytometry/instrumentation , Humans , Jurkat Cells/chemistry , Jurkat Cells/drug effects , Jurkat Cells/pathology , Leukemia, T-Cell/blood , Leukemia, T-Cell/therapy , Necrosis , Photopheresis , Reproducibility of Results , SolutionsABSTRACT
FOXP3 is a unique marker for CD4+CD25+ regulatory T cells (Tregs). In solid tumours, high numbers of Tregs are associated with a poor prognosis. Knowledge about the implications of Tregs for the behaviour of haematological malignancies is limited. In this study, skin biopsies from 86 patients with mycosis fungoides (MF) and cutaneous T-cell lymphoma (CTCL) unspecified were analysed for the expression of FOXP3 on tumour cells and tumour-infiltrating Tregs. Labelling of above 10% of the neoplastic cells was seen in one case classified as an aggressive epidermotropic CD8+ cytotoxic CTCL. In the remaining 85 cases, the atypical neoplastic infiltrate was either FOXP3 negative (n=80) or contained only very occasional weakly positive cells (n=5). By contrast, all biopsies showed varying numbers of strongly FOXP3+ tumour-infiltrating Tregs. MF with early or infiltrated plaques had significantly higher numbers of FOXP3+ Tregs than CTCL unspecified or advanced MF with tumours or transformation to large cell lymphoma. An analysis of all patients demonstrated that increasing numbers of FOXP3+ Tregs were associated with improved survival in both MF and CTCL unspecified. In conclusion, our data indicate that the presence of FOXP3+ Tregs in CTCL is associated with disease stage and patient survival.
Subject(s)
Forkhead Transcription Factors/analysis , Lymphocytes, Tumor-Infiltrating/immunology , Lymphoma, T-Cell, Cutaneous/pathology , Mycosis Fungoides/pathology , Skin Neoplasms/pathology , T-Lymphocytes, Regulatory/immunology , Adult , Aged , Aged, 80 and over , Cell Line, Tumor , Female , Humans , Jurkat Cells/chemistry , Kaplan-Meier Estimate , Lymphocytes, Tumor-Infiltrating/chemistry , Lymphocytes, Tumor-Infiltrating/pathology , Lymphoma, T-Cell, Cutaneous/immunology , Lymphoma, T-Cell, Cutaneous/mortality , Male , Middle Aged , Mycosis Fungoides/mortality , Neoplasm Staging , Prognosis , Proportional Hazards Models , Recombinant Fusion Proteins/analysis , Skin Neoplasms/immunology , Skin Neoplasms/mortality , Survival Analysis , T-Lymphocytes, Regulatory/chemistry , T-Lymphocytes, Regulatory/pathologyABSTRACT
Microfluidic interfaces coupled to ESI mass spectrometers hold great potential for proteomics as they have been shown to augment the overall sensitivity of measurements and require only a minimum of operator manipulations as compared to conventional nano-LC interfaces. Here, we evaluated a new type of HPLC-Chips holding larger enrichment columns (thus an increased sample loading capacity) for gel-free proteome studies. A tryptic digest of a human T-cell proteome was fractionated by strong cation exchange chromatography and selected fractions were analyzed by MS/MS on an IT mass spectrometer using both the new HPLC-Chip as well as a conventional nano-LC-MS/MS interface. Our results indicate that the HPLC-Chip is capable of handling very complex peptide mixtures and, in fact, leads to the identification of more peptides and proteins as compared to when a conventional interface was used. The HPLC-Chip preferentially produced doubly charged tryptic peptides. We further show that MS/MS spectra of doubly charged tryptic peptide ions are more readily identified by MASCOT as compared to those from triply charged precursors and thus argue that besides the improved chromatographic conditions provided by the HPLC-Chip, its peptide charging profile might be a secondary factor leading to an increased proteome coverage.
Subject(s)
Mass Spectrometry , Microfluidic Analytical Techniques , Proteome/analysis , Cell Fractionation , Humans , Jurkat Cells/chemistry , Mass Spectrometry/instrumentation , Mass Spectrometry/methods , Materials Testing , Microfluidic Analytical Techniques/instrumentation , Peptides/analysis , Proteomics/methods , SoftwareSubject(s)
Peptide Fragments/chemistry , Peptide Mapping/methods , Spectrometry, Mass, Electrospray Ionization/methods , Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization/methods , Humans , Jurkat Cells/chemistry , Jurkat Cells/metabolism , Mycobacterium tuberculosis/chemistry , Mycobacterium tuberculosis/metabolism , Proteomics , Salmonella enterica/chemistry , Salmonella enterica/metabolismABSTRACT
Cationic liposomes are used as efficient carriers for gene delivery into mammalian cells due to their ability to bind nucleic acids, adsorb onto the cell surface and fuse with negatively charged membranes. This last property enables the release and escape of their cargo from endosomal compartments. The efficiency of this fusion mainly depends on the surface charge of the target membranes. Here, we report that cells of two different lines, epithelial adenocarcinoma HeLa and lymphocytic leukemia Jurkat T, which externalize PS, are more susceptible to fusion with DOTAP liposomes than control cells. We compared the ability to undergo fusion of untreated and apoptotic cells. Apoptosis was induced by various pro-apoptotic agents and treatments, namely: incubation in the presence of MnCl(2), cytostatic drugs fludarabine and mitoxantrone, staurosporine and serum depletion in the case of HeLa cells. Jurkat T cells were treated similarly except apoptosis was additionally induced by incubation in the presence of 4% EtOH. Epithelial cells fused with the highest efficiencies of lipid mixing, when pretreated with staurosporine. Jurkat T cells were less susceptible to fusion, but they also displayed an increase in fusion efficiency after the induction of apoptosis. Alternatively, we treated the cells with metabolic inhibitors causing ATP-depletion in order to inactivate aminophospholipid translocase. After ATP-depletion, HeLa and Jurkat T cells fused with DOTAP liposomes with higher efficiencies than control cells. Our conclusion is that the lipid asymmetry of natural membranes may limit fusion with cationic liposomes.
Subject(s)
Cell Membrane/chemistry , Fatty Acids, Monounsaturated/chemistry , Fluorescent Dyes/chemistry , Membrane Fusion , Phosphatidylserines/chemistry , Quaternary Ammonium Compounds/chemistry , Antineoplastic Agents/pharmacology , Apoptosis/drug effects , Cell Membrane/drug effects , Chlorides/pharmacology , Enzyme Inhibitors/pharmacology , Fatty Acids, Monounsaturated/metabolism , Fluorescent Dyes/metabolism , HeLa Cells/chemistry , HeLa Cells/drug effects , HeLa Cells/metabolism , Humans , Jurkat Cells/chemistry , Jurkat Cells/drug effects , Jurkat Cells/metabolism , Liposomes , Manganese Compounds/pharmacology , Mitoxantrone/pharmacology , Phosphatidylserines/metabolism , Phospholipid Transfer Proteins/antagonists & inhibitors , Phospholipid Transfer Proteins/metabolism , Quaternary Ammonium Compounds/metabolism , Staurosporine/pharmacology , Vidarabine/analogs & derivatives , Vidarabine/pharmacologyABSTRACT
We have estimated the statistical distribution of the number of plasmids taken up by individual Jurkat lymphoma cells during electroporation in the presence of two plasmids, one encoding for yellow (EYFP) the other for cyan (ECFP) fluorescent protein. The plasmid concentration at which most of the cells take up only one plasmid or several molecules was determined by statistical analysis. We found that cells behaved slightly heterogeneous in plasmid uptake and describe how the homogeneity of a cell population can be quantified by Poisson statistics in order to identify experimental conditions that yield homogeneously transfection-competent cell populations. The experimental procedure worked out with Jurkat cells was applied to assay the effectiveness of antisense RNA in knocking down gene expression in Physarum polycephalum. Double transfection of flagellates with vectors encoding EYFP and antisense-EYFP revealed for the first time that gene expression can be suppressed by co-expression of antisense RNA in Physarum. Quantitative analysis revealed that one copy of antisense expressing gene per EYFP gene was sufficient to completely suppress formation of the EYFP protein in Physarum.
Subject(s)
Gene Expression Regulation , Jurkat Cells/chemistry , Physarum polycephalum/metabolism , Plasmids/genetics , RNA, Antisense/metabolism , Transfection , Animals , Bacterial Proteins/genetics , Bacterial Proteins/metabolism , Electroporation , Eukaryotic Cells/chemistry , Green Fluorescent Proteins/genetics , Green Fluorescent Proteins/metabolism , Humans , Luminescent Proteins/genetics , Luminescent Proteins/metabolism , Physarum polycephalum/genetics , Poisson Distribution , RNA, Messenger/genetics , RNA, Messenger/metabolism , Transformation, GeneticABSTRACT
Mutation or dysregulation of related homeobox genes occurs in leukemia. Using RT-PCR, we screened members of the EHG family of homeobox genes, comprising EN1 (at 2q14), GBX2 (at 2q36), and EN2, GBX1, and HLXB9 (at 7q36), for dysregulation in acute myeloid leukemia (AML) cell lines indicated by chromosomal breakpoints at these sites. Only one EHG-family gene was expressed, HLXB9, in cell line GDM-1 (AML-M4). Karyotypic analysis of GDM-1 revealed a unique t(6;7)(q23;q35), also present in the patient. Fluorescence in situ hybridization analysis showed chromosomal breakpoints close to the region upstream of HLXB9, at 7q36, a region rearranged in certain AML patients, and at 6q23 upstream of MYB, a gene activated in leukemia. Detailed expression analysis suggested ectopic activation of HLXB9 occurred via juxtaposition with regions upstream of MYB, which was highly expressed in GDM-1. Our data identified a cell line model for a novel leukemic translocation involving MYB with HLXB9, further implicating HLXB9 in leukemogenesis.
Subject(s)
Chromosomes, Human, Pair 6/genetics , Chromosomes, Human, Pair 7/genetics , Gene Expression Regulation, Neoplastic/genetics , Genes, myb/physiology , Homeodomain Proteins/genetics , Leukemia, Myelomonocytic, Acute/genetics , Transcription Factors/genetics , Translocation, Genetic/genetics , Cell Line, Tumor , Cytogenetic Analysis/methods , HL-60 Cells/chemistry , HL-60 Cells/metabolism , HeLa Cells/chemistry , HeLa Cells/metabolism , Homeodomain Proteins/physiology , Humans , Jurkat Cells/chemistry , Jurkat Cells/metabolism , K562 Cells/chemistry , K562 Cells/metabolism , Leukemia, Myelomonocytic, Acute/pathology , Proto-Oncogene Proteins c-myb/biosynthesis , Transcription Factors/physiology , U937 Cells/chemistry , U937 Cells/metabolismABSTRACT
In humans, a polymorphic gene encodes the drug-metabolizing enzyme NAT1 (arylamine N-acetyltransferase Type 1), which is widely expressed throughout the body. While the protein-coding region of NAT1 is contained within a single exon, examination of the human EST (expressed sequence tag) database at the NCBI revealed the presence of nine separate exons, eight of which were located in the 5' non-coding region of NAT1. Differential splicing produced at least eight unique mRNA isoforms that could be grouped according to the location of the first exon, which suggested that NAT1 expression occurs from three alternative promoters. Using RT (reverse transcriptase)-PCR, we identified one major transcript in various epithelial cells derived from different tissues. In contrast, multiple transcripts were observed in blood-derived cell lines (CEM, THP-1 and Jurkat), with a novel variant, not identified in the EST database, found in CEM cells only. The major splice variant increased gene expression 9-11-fold in a luciferase reporter assay, while the other isoforms were similar or slightly greater than the control. We examined the upstream region of the most active splice variant in a promoter-reporter assay, and isolated a 257 bp sequence that produced maximal promoter activity. This sequence lacked a TATA box, but contained a consensus Sp1 site and a CAAT box, as well as several other putative transcription-factor-binding sites. Cell-specific expression of the different NAT1 transcripts may contribute to the variation in NAT1 activity in vivo.
Subject(s)
5' Untranslated Regions/genetics , Alternative Splicing/genetics , Arylamine N-Acetyltransferase/genetics , Genome, Human , Isoenzymes/genetics , Promoter Regions, Genetic/genetics , Protein Biosynthesis/genetics , Breast Neoplasms/genetics , Breast Neoplasms/pathology , Carcinoma/genetics , Carcinoma/pathology , Carcinoma, Hepatocellular/genetics , Carcinoma, Hepatocellular/pathology , Cell Line, Tumor , Cloning, Molecular , Exons/genetics , Gene Expression Regulation, Neoplastic/genetics , Genetic Variation/genetics , HT29 Cells/chemistry , HT29 Cells/metabolism , HeLa Cells/chemistry , HeLa Cells/metabolism , Humans , Jurkat Cells/chemistry , Jurkat Cells/metabolism , Leukemia, Lymphoid/genetics , Leukemia, Lymphoid/pathology , Liver Neoplasms/genetics , Liver Neoplasms/pathology , Lung Neoplasms/genetics , Lung Neoplasms/pathology , Melanoma/genetics , Melanoma/pathologyABSTRACT
The ADAM (a disintegrin and metalloprotease) family of proteins possess both proteolytic and adhesive domains. We have established previously that the disintegrin domain of ADAM28, an ADAM expressed by human lymphocytes, is recognized by the integrin alpha4beta1. The present study characterizes the integrin binding properties of the disintegrin-like domains of human ADAM7, ADAM28 and ADAM33 with the integrins alpha4beta1, alpha4beta7 and alpha9beta1. Cell-adhesion assays demonstrated that, similar to ADAM28, the ADAM7 disintegrin domain supported alpha4beta1-dependent Jurkat cell adhesion, whereas the ADAM33 disintegrin domain did not. The lymphocyte integrin alpha4beta7 was also found to recognize both disintegrin domains of ADAM7 and ADAM28, but not of ADAM33. This is the first demonstration that mammalian disintegrins are capable of interacting with alpha4beta7. All three disintegrin domains supported alpha9beta1-dependent cell adhesion. Recognition by both alpha4beta1 and alpha4beta7 of ADAM7 and ADAM28 was activation-dependent, requiring either the presence of Mn2+ or an activating monoclonal antibody for cell attachment. Charge-to-alanine mutagenesis experiments revealed that the same residues within an individual ADAM disintegrin domain function in recognizing multiple integrins. However, the residues within a specific region of each ADAM disintegrin-like domain required for integrin binding were distinct. These results establish that ADAM7 and ADAM28 are recognized by the leucocyte integrins alpha4beta1, alpha4beta7 and alpha9beta1. ADAM33 exclusively supported only alpha9beta1-dependent adhesion.
Subject(s)
Integrin alpha4beta1/metabolism , Integrins/metabolism , Lymphocytes/metabolism , Membrane Glycoproteins/metabolism , Metalloendopeptidases/metabolism , ADAM Proteins , Amino Acid Sequence , Cell Adhesion/physiology , Cell Line, Tumor , Humans , Jurkat Cells/chemistry , Jurkat Cells/metabolism , K562 Cells/chemistry , K562 Cells/metabolism , Molecular Sequence Data , Peptides/chemistry , Peptides/metabolism , Protein Structure, Tertiary , Receptors, Lymphocyte Homing/metabolism , Sequence Homology, Amino AcidABSTRACT
To assess the effects of inflammation on the generation of circulating DNA from dead and dying cells, plasma DNA levels were determined in BALB/c mice, administered apoptotic or necrotic Jurkat cells following induction of peritonitis by treatment with thioglycollate (TG), peptone (PT), or sodium periodate (NaIO(4)). In mice receiving TG or NaIO(4), plasma DNA levels following intraperitoneal administration of Jurkat cells were significantly reduced compared with controls, whereas they were not affected in mice receiving PT. To determine the basis of these differences, the cellular composition of peritoneal fluids prior to the administration of the dead cells was analyzed. Among agents tested, TG administration led to the largest increase in cells, both neutrophils and monocytes. As shown by flow cytometry, the exudates contained apoptotic neutrophils and macrophages, with the highest levels in the TG-induced exudates. Analysis of DNA and caspase 3 in the fluids also showed differences. TG exudates showed increases in DNA and caspase 3, while NaIO(4)-induced exudates had an increase only in DNA. Fluid from PT-treated mice did not have increases in DNA or caspase 3. Together, these results indicate that prior inflammation can affect the generation of blood DNA from apoptotic or necrotic cells, although this effect may vary depending on the composition of the exudates with respect to cells as well as DNA.
Subject(s)
Apoptosis/physiology , DNA/blood , Inflammation/physiopathology , Peritoneum/chemistry , Animals , Cells/chemistry , Cells/immunology , Cells/metabolism , DNA/chemistry , DNA/drug effects , Female , Humans , Inflammation/metabolism , Jurkat Cells/chemistry , Mice , Mice, Inbred BALB C , Peptones/chemistry , Peptones/pharmacology , Periodic Acid/chemistry , Periodic Acid/pharmacology , Peritonitis/chemically induced , Thioglycolates/chemistry , Thioglycolates/pharmacology , Time FactorsABSTRACT
Paclitaxel (PTX), a microtubule-active drug, causes mitotic arrest leading to apoptosis in certain tumor cell lines. Here we investigated the effects of PTX on human arterial smooth muscle cell (SMC) cells. In SMC, PTX caused both (a) primary arrest in G(1) and (b) post-mitotic arrest in G(1). Post-mitotic cells were multinucleated (MN) with either 2C (near-diploid) or 4C (tetraploid) DNA content. At PTX concentrations above 12 ng/ml, MN cells had 4C DNA content consistent with the lack of cytokinesis during abortive mitosis. Treatment with 6-12 ng/ml PTX yielded MN cells with 2C DNA content. Finally, 1-6 ng/ml of PTX, the lowest concentrations that affected cell proliferation, caused G(1) arrest without multinucleation. It is important that PTX did not cause apoptosis in SMC. The absence of apoptosis could be explained by mitotic exit and G(1) arrest as well as by low constitutive levels of caspase expression and by p53 and p21 induction. Thus, following transient mitotic arrest, SMC exit mitosis to form MN cells. These post-mitotic cells were subsequently arrested in G(1) but maintained normal elongated morphology and were viable for at least 21 days. We conclude that in SMC PTX causes post-mitotic cell cycle arrest rather than cell death.
Subject(s)
G1 Phase/drug effects , Muscle, Smooth, Vascular/cytology , Myocytes, Smooth Muscle/drug effects , Paclitaxel/pharmacology , Aorta/cytology , Apoptosis/drug effects , Cell Count , Cell Line , Cell Proliferation/drug effects , Cell Survival/drug effects , Cell Survival/physiology , Coronary Vessels/cytology , HL-60 Cells/chemistry , HL-60 Cells/metabolism , HL-60 Cells/pathology , Humans , Jurkat Cells/chemistry , Jurkat Cells/metabolism , Jurkat Cells/pathology , Mitosis/drug effects , Muscle, Smooth, Vascular/drug effects , Ploidies , Proto-Oncogene Proteins p21(ras)/metabolismABSTRACT
In this report, we have achieved a richer view of the transcriptome for Chromosomes 21 and 22 by using high-density oligonucleotide arrays on cytosolic poly(A)(+) RNA. Conservatively, only 31.4% of the observed transcribed nucleotides correspond to well-annotated genes, whereas an additional 4.8% and 14.7% correspond to mRNAs and ESTs, respectively. Approximately 85% of the known exons were detected, and up to 21% of known genes have only a single isoform based on exon-skipping alternative expression. Overall, the expression of the well-characterized exons falls predominately into two categories, uniquely or ubiquitously expressed with an identifiable proportion of antisense transcripts. The remaining observed transcription (49.0%) was outside of any known annotation. These novel transcripts appear to be more cell-line-specific and have lower and less variation in expression than the well-characterized genes. Novel transcripts were further characterized based on their distance to annotations, transcript size, coding capacity, and identification as antisense to intronic sequences. By RT-PCR, 126 novel transcripts were independently verified, resulting in a 65% verification rate. These observations strongly support the argument for a re-evaluation of the total number of human genes and an alternative term for "gene" to encompass these growing, novel classes of RNA transcripts in the human genome.
Subject(s)
Chromosomes, Human, Pair 21/genetics , Chromosomes, Human, Pair 22/genetics , RNA/genetics , Transcription, Genetic/genetics , Cell Line , Cell Line, Tumor , Chromosome Mapping/methods , DNA, Neoplasm/genetics , Gene Expression Profiling/methods , Genes/genetics , Genes, Neoplasm/genetics , Humans , Jurkat Cells/chemistry , Jurkat Cells/metabolism , Molecular Sequence Data , Oligonucleotide Array Sequence Analysis/methods , Oligonucleotide Probes/genetics , RNA, Messenger/geneticsABSTRACT
Leukemias are considered malignant clonal disorders arising from the accumulation of mutations in hematopoietic cells; the majority of these mutations are thought to be acquired somatically. Measurement of mutation frequency (Mf) at the hypoxanthine phosphoribosyltransferase (HPRT) locus has been developed as a method for estimating genomic instability. We investigated the Mf in 16 leukemic cell lines to determine whether these cell lines showed evidence of genomic instability. Although some leukemic cell lines had markedly elevated Mfs, the Mfs at the HPRT locus in leukemic cell lines were not always higher than those of B-lymphoblastoid cell lines and T lymphocytes from normal individuals. We were able to identify the HPRT mutation for 159 of 160 individual HPRT mutants. The HPRT mutations were characterized at a molecular level and classified as either gross chromosomal rearrangements (GCRs) or point mutations, such as single-nucleotide substitutions, insertions, or deletions. With rare exceptions, individual leukemic cell lines showed either point mutations or GCR, but not both. Of note, all the cell lines that primarily showed point mutations are known to be defective in mismatch repair machinery.
Subject(s)
Hypoxanthine Phosphoribosyltransferase/genetics , Leukemia/genetics , Mutation/genetics , Adolescent , Adult , Aged , B-Lymphocytes/chemistry , B-Lymphocytes/metabolism , B-Lymphocytes/pathology , Cell Line, Tumor , Child , Child, Preschool , DNA Mutational Analysis/methods , Female , Genetic Markers/genetics , Genomic Instability/genetics , HL-60 Cells/chemistry , HL-60 Cells/metabolism , Humans , Jurkat Cells/chemistry , Jurkat Cells/metabolism , K562 Cells/chemistry , K562 Cells/metabolism , Leukemia/pathology , Male , Mutagenesis/genetics , Pilot Projects , RNA Splicing/genetics , RNA, Messenger/metabolism , RNA, Neoplasm/genetics , Recombination, Genetic/genetics , U937 Cells/chemistry , U937 Cells/metabolismABSTRACT
The t(9;11) has been described in patients with acute myeloid leukemia (AML), and two genes [AF9 (at 9p21) and FBP17 (at 9q34)] have been cloned as fusion partners of the MLL gene. From an AML-M5 with a t(9;11)(q34;q23), we identified a novel MLL fusion partner, AF9Q34. The AF9Q34 protein shows high homology with nGAP, a RAS GTPase-activating protein (RASGAP), and contains the highly conserved GRD and FLR motifs characteristic of RASGAPs. Recently, the rat homologue (DAB2IP) also was identified and reported to act as a RASGAP both in vivo and in vitro. RASGAPs negatively regulate the activity of RAS proteins that modulate diverse cellular processes by cycling between an inactive GDP-bound and an active GTP-bound state. In addition, the NH(2) terminus harbors an amino acid stretch with homology to the pleckstrin homology (PH) domain implicated in regulating the interaction between RAS and the catalytic domain of RASGAP. As a result of the breakpoint in the AF9Q34-MLL fusion protein, this PH domain is disrupted. This suggests that because of the translocation, the normal function of the AF9Q34 gene is aborted. Thus, AF9Q34 encodes a novel RASGAP gene that appears to be deregulated as a result of the translocation. The identification of this RASGAP protein in a novel MLL fusion implies that an indirect RAS-deregulating mechanism could be involved in leukemic transformation.
