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Titlebook: Disease Gene Identification; Methods and Protocol Johanna K.‘DiStefano Book 2018Latest edition Springer Science+Business Media, LLC 2018 bi

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Using Fluidigm C1 to Generate Single-Cell Full-Length cDNA Libraries for mRNA Sequencings confirmation of the presence of a ., . cell and recording of phenotypic information, quality control measures that are crucial for streamlining downstream data processing and enhancing overall data validity.
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Optimized Methodology for the Generation of RNA-Sequencing Libraries from Low-Input Starting Materialications, such as flow cytometry-sorted cells and clinical specimens, due to protocol advances enabling the use of very low input material ranging from 10 pg to 10 ng of total RNA or 1–1000 intact cells. In this chapter, we present an optimized and detailed approach to RNA-seq for use with low abundance samples.
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Kristian Dahl Hertz,Philip Haldingbalance between the ability to recapitulate many aspects of human disease, while still offering an abundance of powerful cell biological, genetic, and genomic tools for disease gene discovery. . and other nonmammalian models have produced, and will continue to produce, key insights into human disease pathogenesis.
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