Literature DB >> 22951961

Development of the "Three-step MACS": a novel strategy for isolating rare cell populations in the absence of known cell surface markers from complex animal tissue.

Mathia Y Lee1, Thomas Lufkin.   

Abstract

To circumvent the difficulty of isolating specific cell populations by MACS from dissociated complex animal tissue, when their proportions reached levels similar to that of the background, we developed the "Three-step MACS" strategy. Cells of interest are defined by their expression of a particular gene(s) of interest rather by than their natural cell surface markers or size. A two-component transgenic cell surface protein, for two sequential rounds of MACS, is expressed under the promoter control of the endogenous gene of interest by means of gene targeting and the generation of transgenic tissue. An initial step to remove dead cells is also used. Here, we describe proof-of-concept experiments, using the biotin acceptor peptide (BAP)-low-affinity nerve growth factor receptor as the two-component protein. The first component, the BAP, can be biotinylated in specific subsets of cells expressing a particular gene by expressing the biotinylating enzyme, hBirA = humanized BirA (hBirA), under the promoter control of another gene defining the specific subpopulation. We showed that a rare population of cells (1.1% of the 13.5 days postcoital mouse embryo) could be enriched to a sufficiently high purity (84.4%). From another sample with 0.1% of our cells of interest, we achieved a 40.3% pure sample. The low cost, speed, and technical ease of the Three-step MACS also make it scalable and hence, an ideal method for preparing sufficient quantities of biological samples for sensitive, high-throughput assays.

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Year:  2012        PMID: 22951961      PMCID: PMC3336840          DOI: 10.7171/jbt.12-2302-003

Source DB:  PubMed          Journal:  J Biomol Tech        ISSN: 1524-0215


  48 in total

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3.  Side population cells isolated from different tissues share transcriptome signatures and express tissue-specific markers.

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4.  High gradient magnetic cell separation with MACS.

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5.  Genome-wide expression profiling; a panel of mouse tissues discloses novel biological functions of liver X receptors in adrenals.

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Journal:  Eur J Haematol       Date:  1994-05       Impact factor: 2.997

7.  Simple affinity purification of antibodies using in vivo biotinylation of a fusion protein.

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Authors:  S Kawauchi; S Takahashi; O Nakajima; H Ogino; M Morita; M Nishizawa; K Yasuda; M Yamamoto
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Journal:  Prenat Diagn       Date:  1994-12       Impact factor: 3.050

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6.  Antibody-free magnetic cell sorting of genetically modified primary human CD4+ T cells by one-step streptavidin affinity purification.

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7.  In vivo genome-wide analysis of multiple tissues identifies gene regulatory networks, novel functions and downstream regulatory genes for Bapx1 and its co-regulation with Sox9 in the mammalian vertebral column.

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9.  Expression of Tmem119/Sall1 and Ccr2/CD69 in FACS-Sorted Microglia- and Monocyte/Macrophage-Enriched Cell Populations After Intracerebral Hemorrhage.

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Review 10.  Strategies for enrichment of circulating tumor cells.

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