Gary de Jong scite author profile

Telomeres have emerged as crucial cellular elements in aging and various diseases including cancer. To measure the average length of telomere repeats in cells, we describe our protocols that use fluorescent in situ hybridization (FISH) with labeled peptide nucleic acid (PNA) probes specific for telomere repeats in combination with fluorescence measurements by flow cytometry (flow FISH). Flow FISH analysis can be performed using commercially available flow cytometers, and has the unique advantage over other methods for measuring telomere length of providing multi-parameter information on the length of telomere repeats in thousands of individual cells. The accuracy and reproducibility of the measurements is augmented by the automation of most pipetting (aspiration and dispensing) steps, and by including an internal standard (control cells) with a known telomere length in every tube. The basic protocol for the analysis of nucleated blood cells from 22 different individuals takes about 12 h spread over 2-3 days.

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Flow-Cytometric Confirmation of Aneuploidy in Sperm from Triploid Rainbow Trout

Benfey

Solar

Jong

et al. 1986

Transactions of the American Fisheries Society

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Triploid rainbow trout Salmo gairdneri produce spermatozoa with DNA contents intermediate between haploid and diploid values. This confirms that these spermatozoa are aneuploid and explains why progeny produced from the fertilization of haploid eggs with such sperm are not viable. Triploid males have significantly lower spermatocrit and smaller testes than diploids, but still develop normal secondary sexual characteristics and exhibit postspawning mortality.

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Prolactin-Regulated Apoptosis of Nb2 Lymphoma Cells: pim-1 , bcl-2 , and bax Expression

Krumenacker

Buckley

Leff

et al. 1998

ENDO

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Lactogen-dependent Nb2 lymphoma cells, widely employed for studying prolactin (PRL) mitogenic mechanisms, are also useful for investigations of apoptosis in T-lineage lymphocytes. Utilizing PRL-dependent Nb2-11 cultures, apoptosis-regulatory genes were evaluated for participation in dexamethasone- (DEX) provoked cell death or its inhibition by PRL. Treatment of lactogen-starved, G1-arrested Nb2-11 cells with DEX (100 nM) activated apoptosis within 12 h evaluated by flow cytometric analysis of fragmented DNA. This effect was not associated with altered expression of bcl-2, bax, or pim-1. PRL (10 ng/mL), coincubated with DEX-treated cells, completely blocked DEX-induced apoptosis. This inhibition was associated with increased expression of bcl-2 and pim-1 mRNAs, genes reported to suppress apoptosis, within 2-6 h after addition of the hormone. Moreover, the increased transcription of bcl-2 and pim-1 was coupled to increases in their protein levels. The results suggest that bcl-2, bax, and pim-1 do not play a critical role in DEX-induced apoptosis in Nb2 cells. However, expression of bcl-2, together with pim-1, may have a role in mediating the antiapoptotic actions of PRL.

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Flow Cytometry of Mitotic Cells

Anderson

Jong

Vincent

et al. 1998

Experimental Cell Research

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Efficient transfer of chromosome-based DNA constructs into mammalian cells

Oberle

Jong²,

Drayer³

et al. 2004

Biochimica et Biophysica Acta (BBA) - Gene Structure and Expres

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Gary de Jong

Flow cytometry and FISH to measure the average length of telomeres (flow FISH)

Flow-Cytometric Confirmation of Aneuploidy in Sperm from Triploid Rainbow Trout

Prolactin-Regulated Apoptosis of Nb2 Lymphoma Cells: pim-1 , bcl-2 , and bax Expression

Flow Cytometry of Mitotic Cells

Efficient transfer of chromosome-based DNA constructs into mammalian cells

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