ABSTRACT
Determining mechanisms of drug action in human cells remains a major challenge. Here we describe an approach in which multiple-drug-resistant clones are isolated and transcriptome sequencing is used to find mutations in each clone. Further analysis of mutations common to more than one clone can identify a drug's physiological target and indirect resistance mechanisms, as indicated by our proof-of-concept studies of the cytotoxic anticancer drugs BI 2536 and bortezomib.
Subject(s)
Antineoplastic Agents/pharmacology , Cell Cycle Proteins/antagonists & inhibitors , Cell Cycle Proteins/genetics , Drug Resistance, Neoplasm/genetics , Protein Serine-Threonine Kinases/antagonists & inhibitors , Protein Serine-Threonine Kinases/genetics , Proto-Oncogene Proteins/antagonists & inhibitors , Proto-Oncogene Proteins/genetics , Sequence Analysis, DNA , Transcriptome/genetics , Antineoplastic Agents/chemistry , Boronic Acids/chemistry , Boronic Acids/pharmacology , Bortezomib , Cell Line, Tumor , Drug Resistance, Neoplasm/drug effects , Humans , Pteridines/chemistry , Pteridines/pharmacology , Pyrazines/chemistry , Pyrazines/pharmacology , Polo-Like Kinase 1ABSTRACT
Telomere length homeostasis is achieved by a balance of telomere shortening caused by DNA replication and nucleolytic attack and telomere lengthening by telomerase. The importance of telomere length maintenance to human health is best illustrated by dyskeratosis congenita (DC) a disease of telomere shortening caused by mutations in telomerase subunits. DC patients suffer stem cell depletion and die of bone marrow stem cell failure. Recently a new class of particularly severe DC patients was found to harbor mutations in the shelterin subunit TIN2. The DC-TIN2 mutations were clustered in small domain of unknown function. In a recently published study we showed that the DC mutation cluster in TIN2 harbored a binding site for heterochromatin protein 1 (HP1) and further, that HP1 binding to TIN2 was required for sister telomere cohesion in S phase and for telomere length maintenance by telomerase. We briefly review and discuss the implications of our findings in this Extra View, and present some new data that may shed light on how sister telomere cohesion could influence telomere elongation by telomerase.
Subject(s)
Telomerase/metabolism , Telomere/metabolism , Binding Sites , Cell Line, Tumor , Chromobox Protein Homolog 5 , Chromosomal Proteins, Non-Histone/metabolism , Dyskeratosis Congenita/enzymology , Dyskeratosis Congenita/metabolism , Dyskeratosis Congenita/pathology , Humans , Mutation , Protein Binding , S Phase , Telomerase/genetics , Telomere/genetics , Telomere Homeostasis , Telomere Shortening , Telomere-Binding Proteins/genetics , Telomere-Binding Proteins/metabolismABSTRACT
Human telomere function is mediated by shelterin, a six-subunit complex that is required for telomere replication, protection, and cohesion. TIN2, the central component of shelterin, has binding sites to three subunits: TRF1, TRF2, and TPP1. Here we identify a fourth partner, heterochromatin protein 1γ (HP1γ), that binds to a conserved canonical HP1-binding motif, PXVXL, in the C-terminal domain of TIN2. We show that HP1γ localizes to telomeres in S phase, where it is required to establish/maintain cohesion. We further demonstrate that the HP1-binding site in TIN2 is required for sister telomere cohesion and can impact telomere length maintenance by telomerase. Remarkably, the PTVML HP1-binding site is embedded in the recently identified cluster of mutations in TIN2 that gives rise to dyskeratosis congenita (DC), an inherited bone marrow failure syndrome caused by defects in telomere maintenance. We show that DC-associated mutations in TIN2 abrogate binding to HP1γ and that DC patient cells are defective in sister telomere cohesion. Our data indicate a novel requirement for HP1γ in the establishment/maintenance of cohesion at human telomeres and, furthermore, may provide insight into the mechanism of pathogenesis in TIN2-mediated DC.
Subject(s)
Chromosomal Proteins, Non-Histone/metabolism , Telomere/metabolism , Amino Acid Sequence , Cell Line , Chromobox Protein Homolog 5 , Dyskeratosis Congenita/genetics , HeLa Cells , Humans , Male , Molecular Sequence Data , Mutation/genetics , Protein Binding/genetics , S Phase/genetics , Shelterin Complex , Telomerase/metabolism , Telomere/genetics , Telomere-Binding Proteins/chemistry , Telomere-Binding Proteins/genetics , Telomere-Binding Proteins/metabolismABSTRACT
INTRODUCTION: Fluorescent speckle microscopy (FSM) is a live imaging and quantitative measurement technique used for analyzing motion and turnover of macromolecular assemblies in vivo and in vitro. It differs from related imaging techniques such as photobleaching and photoactivation in its use of substantially lower concentrations of fluorescently labeled assembly subunits. When small numbers of labeled subunits and large numbers of unlabeled subunits become randomly incorporated together into a macromolecular structure, the random distribution of fluorophores generates nonuniform fluorescence intensity patterns that appear as distinct puncta against low background fluorescence. These puncta, called speckles, serve as fiduciary markers so that motion and turnover of the structure are visualized. Computational analysis of speckle image data transforms FSM into a powerful tool for high-resolution quantitative analysis of macromolecular assembly dynamics. Successful application of FSM depends on the ability to reliably generate and image speckles, which are characterized by their weak emission signals, and to effectively extract quantitative information through computational analysis of speckle image data, which are characterized by their stochastic fluctuations, low signal-to-noise ratios, and high spatiotemporal complexity. This article aims to provide a practical introduction to basic principles, experimental implementation, and computational data analysis of FSM. Examples are used to show the application of FSM in analyzing the dynamic organization and assembly/disassembly of cytoskeletal filament networks, an area in which FSM analysis has found great success.
Subject(s)
Cytological Techniques/methods , Image Processing, Computer-Assisted/methods , Macromolecular Substances/metabolism , Microscopy, Fluorescence/methods , Fluorescent Dyes , Staining and Labeling/methods , Time-Lapse Imaging/methodsABSTRACT
Accuracy in chromosome segregation depends on the assembly of a bipolar spindle. Unlike mitotic spindles, which have roughly equal amounts of kinetochore microtubules (kMTs) and nonkinetochore microtubules (non-kMTs), vertebrate meiotic spindles are predominantly comprised of non-kMTs, a large subset of which forms an antiparallel "barrel" array at the spindle equator. Though kMTs are needed to drive chromosome segregation, the contributions of non-kMTs are more mysterious. Here, we show that increasing the concentration of Op18/stathmin, a component of the chromosome-mediated microtubule formation pathway that directly controls microtubule dynamics, can be used to deplete non-kMTs in the vertebrate meiotic spindle assembled in Xenopus egg extracts. Under these conditions, kMTs and the spindle pole-associated non-kMT arrays persist in smaller spindles. In excess Op18, distances between sister kinetochores, an indicator of tension across centromeres, remain unchanged, even though kMTs flux poleward with a approximately 30% slower velocity, and chromosomes oscillate more than in control metaphase spindles. Remarkably, kinesin-5, a conserved motor protein that can push microtubules apart and is required for the assembly and maintenance of bipolar meiotic spindles, is not needed to maintain spindle bipolarity in the presence of excess Op18. Our data suggest that non-kMTs in meiotic spindles contribute to normal kMT dynamics, stable chromosome positioning, and the establishment of proper spindle size. We propose that without non-kMTs, metaphase meiotic spindles are similar to mammalian mitotic spindles, which balance forces to maintain metaphase spindle organization in the absence of extensive antiparallel microtubule overlap at the spindle equator or a key mitotic kinesin.
Subject(s)
Chromosome Segregation/physiology , Meiosis/physiology , Microtubules/physiology , Spindle Apparatus/physiology , Stathmin/metabolism , Animals , Flow Cytometry , Kinesins/metabolism , Microscopy, Fluorescence , Xenopus laevisABSTRACT
Bipolarity of the meiotic spindle, required for proper chromosome segregation, is maintained throughout cell division despite rapid microtubule turnover. How this is achieved has remained mysterious, as determining the organization of individual spindle microtubules has been difficult. Here, we develop single-fluorophore speckle imaging to examine microtubule organization in the vertebrate meiotic spindle. We find that the mean length of microtubules is approximately 40% of spindle length. Long and short filaments distribute randomly throughout the spindle and those in close proximity can move in the same direction with highly heterogeneous velocities. The ratio between microtubule and spindle lengths remains unchanged as spindles elongate upon dynein-dynactin inhibition. However, maintaining this ratio depends on proper kinesin-5 function. Our data suggest that force transmission within the spindle must be understood in terms of the crosslinking dynamics of a tiled array of individual filaments, most of which do not span the distance from the pole to the metaphase plate.
Subject(s)
Fluorescent Dyes , Luminescent Measurements/methods , Meiosis , Microtubules/chemistry , Spindle Apparatus/chemistry , Animals , Fluorescent Dyes/chemistry , Hydrazines/chemistry , Microtubules/physiology , Microtubules/ultrastructure , Spindle Apparatus/physiology , Spindle Apparatus/ultrastructure , XenopusABSTRACT
Previous studies in human cells indicate that sister telomeres have distinct requirements for their separation at mitosis. In cells depleted for tankyrase 1, a telomeric poly(ADP-ribose) polymerase, sister chromatid arms and centromeres separate normally, but telomeres remain associated and cells arrest in mitosis. Here, we use biochemical and genetic approaches to identify proteins that might mediate the persistent association at sister telomeres. We use immunoprecipitation analysis to show that the telomeric proteins, TRF1 (an acceptor of PARsylation by tankyrase 1) and TIN2 (a TRF1 binding partner) each bind to the SA1 ortholog of the cohesin Scc3 subunit. Sucrose gradient sedimentation shows that TRF1 cosediments with the SA1-cohesin complex. Depletion of the SA1 cohesin subunit or the telomeric proteins (TRF1 and TIN2) restores the normal resolution of sister telomeres in mitosis in tankyrase 1-depleted cells. Moreover, depletion of TRF1 and TIN2 or SA1 abrogates the requirement for tankyrase 1 in mitotic progression. Our studies indicate that sister telomere association in human cells is mediated by a novel association between a cohesin subunit and components of telomeric chromatin.
Subject(s)
Telomere/ultrastructure , Cell Cycle Proteins/metabolism , Centrifugation, Density Gradient , Chromosomal Proteins, Non-Histone/metabolism , Gene Expression Regulation, Neoplastic , HeLa Cells , Humans , Immunoprecipitation , In Situ Hybridization, Fluorescence , Mitosis , Models, Biological , Nuclear Proteins/metabolism , Poly(ADP-ribose) Polymerases/metabolism , Protein Binding , Tankyrases/genetics , Tankyrases/metabolism , Telomere-Binding Proteins/metabolism , Telomeric Repeat Binding Protein 1/metabolism , CohesinsABSTRACT
BACKGROUND: Human telomeres are coated by the telomere repeat binding proteins TRF1 and TRF2, which are believed to function independently to regulate telomere length and protect chromosome ends, respectively. RESULTS: Here, we show that TRF1 and TRF2 are linked via TIN2, a previously identified TRF1-interacting protein, and its novel binding partner TINT1. TINT1 localized to telomeres via TIN2, where it functioned as a negative regulator of telomerase-mediated telomere elongation. TIN2 associated with TINT1, and TRF1 or TRF2 throughout the cell cycle, revealing a partially redundant unit in telomeric chromatin that may provide flexibility in telomere length control. Indeed, when TRF1 was removed from telomeres by overexpression of the positive telomere length regulator tankyrase 1, the TIN2/TINT1 complex remained on telomeres via an increased association with TRF2. CONCLUSIONS: Our findings suggest a dynamic cross talk between TRF1 and TRF2 and provide a molecular mechanism for telomere length homeostasis by TRF2 in the absence of TRF1.
