A Translational Profiling Approach for the Molecular Characterization of CNS Cell Types

Heiman, Myriam; Schaefer, Anne; Gong, Shiaoching; Peterson, Jayms D.; Day, Michelle; Ramsey, Keri; Suárez‐Fariñas, Mayte; Schwarz, Cordelia S.; Stephan, Dietrich A.; Surmeier, D. James; Greengard, Paul; Heintz, Nathaniel

doi:10.1016/j.cell.2008.10.028

Cited by 1,059 publications

(1,179 citation statements)

References 56 publications

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“…TRAP followed a detailed protocol supplied by the Dr. N. Heintz laboratory at the Rockefeller University (New York, New York, USA) (19,20). Kidneys were removed 24 hours after surgery.…”

Section: Methodsmentioning

confidence: 99%

“…Recently, translating ribosome affinity purification (TRAP) has been developed to identify cell type-specific changes in mRNA populations at the whole-organ level (19,20). A driver for development of TRAP technology has been the need to obtain molecular signatures for adult neuronal types where recovery of intact cells is not possible through tissue dissociation and FACS.…”

Section: Introductionmentioning

confidence: 99%

“…A driver for development of TRAP technology has been the need to obtain molecular signatures for adult neuronal types where recovery of intact cells is not possible through tissue dissociation and FACS. In TRAP, an EGFP-tagged form of the L10a ribosomal subunit (EGFP-L10a) is activated within a cell type of interest (19,20). The profile of ribosome-bound mRNAs in the cell type is determined by affinity purification of ribosomes from a whole-organ lysate with anti-EGFP antibodies, followed by microarray profiling or sequencing of stripped mRNAs.…”

Section: Introductionmentioning

confidence: 99%

“…The neural TRAP studies have used large BACs carrying cell type-specific regulatory information to drive an EGFP-L10a expression cassette within neural cell types of interest (19,20). Recently, reports in Drosophila, Xenopus laevis, and zebrafish emphasize the utility of the approach (21)(22)(23).…”

Section: Introductionmentioning

confidence: 99%

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Cell-specific translational profiling in acute kidney injury

et al. 2014

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Acute kidney injury (AKI) promotes an abrupt loss of kidney function that results in substantial morbidity and mortality. Considerable effort has gone toward identification of diagnostic biomarkers and analysis of AKI-associated molecular events; however, most studies have adopted organ-wide approaches and have not elucidated the interplay among different cell types involved in AKI pathophysiology. To better characterize AKI-associated molecular and cellular events, we developed a mouse line that enables the identification of translational profiles in specific cell types. This strategy relies on CRE recombinase-dependent activation of an EGFP-tagged L10a ribosomal protein subunit, which allows translating ribosome affinity purification (TRAP) of mRNA populations in CRE-expressing cells. Combining this mouse line with cell type-specific CRE-driver lines, we identified distinct cellular responses in an ischemia reperfusion injury (IRI) model of AKI. Twenty-four hours following IRI, distinct translational signatures were identified in the nephron, kidney interstitial cell populations, vascular endothelium, and macrophages/monocytes. Furthermore, TRAP captured known IRI-associated markers, validating this approach. Biological function annotation, canonical pathway analysis, and in situ analysis of identified response genes provided insight into cell-specific injury signatures. Our study provides a deep, cell-based view of early injury-associated molecular events in AKI and documents a versatile, genetic tool to monitor cell-specific and temporal-specific biological processes in disease modeling.

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“…TRAP followed a detailed protocol supplied by the Dr. N. Heintz laboratory at the Rockefeller University (New York, New York, USA) (19,20). Kidneys were removed 24 hours after surgery.…”

Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Cell-specific translational profiling in acute kidney injury

et al. 2014

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“…In wild-type cultured hippocampal neurons expressing DTR-GFP fusion, administration of DT triggered apoptosis of GFP-positive cells (Supplementary Figure S1A). To specifically ablate striatonigral MSNs, we chose to drive the expression of the DTR-GFP construct under the control of a highly enriched striatonigral MSNs gene, Slc35d3 (Heiman et al, 2008;Lobo et al, 2006), using the BAC-based strategy (Supplementary Figure S1B). Transgenic mice were generated by injecting the recombined BAC into the pronuclei of hybrid C57Bl/ 6 Â CB1 F1 fertilized oocytes, which were then implanted into pseudopregnant females.…”

Section: Generation Of Slc35d3 Dtr-gfp Transgenic Micementioning

confidence: 99%

Cellular and Behavioral Outcomes of Dorsal Striatonigral Neuron Ablation: New Insights into Striatal Functions

Révy

Jaouen

Salin

et al. 2014

Neuropsychopharmacol

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The striatum is the input structure of the basal ganglia network that contains heterogeneous neuronal populations, including two populations of projecting neurons called the medium spiny neurons (MSNs), and different types of interneurons. We developed a transgenic mouse model enabling inducible ablation of the striatonigral MSNs constituting the direct pathway by expressing the human diphtheria toxin (DT) receptor under the control of the Slc35d3 gene promoter, a gene enriched in striatonigral MSNs. DT injection into the striatum triggered selective elimination of the majority of striatonigral MSNs. DT-mediated ablation of striatonigral MSNs caused selective loss of cholinergic interneurons in the dorsal striatum but not in the ventral striatum (nucleus accumbens), suggesting a regionspecific critical role of the direct pathway in striatal cholinergic neuron homeostasis. Mice with DT injection into the dorsal striatum showed altered basal and cocaine-induced locomotion and dramatic reduction of L-DOPA-induced dyskinesia in the parkinsonian condition. In addition, these mice exhibited reduced anxiety, revealing a role of the dorsal striatum in the modulation of behaviors involving an emotional component, behaviors generally associated with limbic structures. Altogether, these results highlight the implication of the direct striatonigral pathway in the regulation of heterogeneous functions from cell survival to regulation of motor and emotion-associated behaviors.

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Genome‐Wide Annotation and Quantitation of Translation by Ribosome Profiling

Ingolia

Brar

Rouskin

et al. 2013

CP Molecular Biology

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Recent studies highlight the importance of translational control in determining protein abundance, underscoring the value of measuring gene expression at the level of translation. We present a protocol for genome-wide, quantitative analysis of in vivo translation by deep sequencing. This ribosome profiling approach maps the exact positions of ribosomes on transcripts by nuclease footprinting. The nuclease-protected mRNA fragments are converted into a DNA library suitable for deep sequencing using a strategy that minimizes bias. The abundance of different footprint fragments in deep sequencing data reports on the amount of translation of a gene. Additionally, footprints reveal the exact regions of the transcriptome that are translated. To better define translated reading frames, we describe an adaptation that reveals the sites of translation initiation by pre-treating cells with harringtonine to immobilize initiating ribosomes. The protocol we describe requires 5 – 7 days to generate a completed ribosome profiling sequencing library. Sequencing and data analysis requires a further 4 – 5 days.

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A Translational Profiling Approach for the Molecular Characterization of CNS Cell Types

Cited by 1,059 publications

References 56 publications

Cell-specific translational profiling in acute kidney injury

Cell-specific translational profiling in acute kidney injury

Cellular and Behavioral Outcomes of Dorsal Striatonigral Neuron Ablation: New Insights into Striatal Functions

Genome‐Wide Annotation and Quantitation of Translation by Ribosome Profiling

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