4.6 Article

Characterization of axolotl lampbrush chromosomes by fluorescence in situ hybridization and immunostaining

Journal

EXPERIMENTAL CELL RESEARCH
Volume 401, Issue 2, Pages -

Publisher

ELSEVIER INC
DOI: 10.1016/j.yexcr.2021.112523

Keywords

Axolotl; Ambystoma mexicanum; Lampbrush chromosomes; Centromere; BAC FISH

Funding

  1. National Institute of General Medical Sciences of the National Institutes of Health [R01 GM33397]
  2. National Institutes of Health [R24 RR016344, R24 OD010435, P40OD019794]
  3. Department of Defense [W911NF1110475]

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This study identified 9 lampbrush chromosomes in the oocytes of the Mexican axolotl using RNAseq and BAC probes, and developed a centromere probe that localizes to all 14 centromeres. The measurement of relative LBC arm lengths and RNA polymerase III localization patterns enabled the identification of all LBCs. The data from this study will facilitate a more detailed transcription analysis of individual LBC loops.
The lampbrush chromosomes (LBCs) in oocytes of the Mexican axolotl (Ambystoma mexicanum) were identified some time ago by their relative lengths and predicted centromeres, but they have never been associated completely with the mitotic karyotype, linkage maps or genome assembly. We identified 9 of the axolotl LBCs using RNAseq to identify actively transcribed genes and 13 BAC (bacterial artificial clone) probes containing pieces of active genes. Using read coverage analysis to find candidate centromere sequences, we developed a centromere probe that localizes to all 14 centromeres. Measurements of relative LBC arm lengths and polymerase III localization patterns enabled us to identify all LBCs. This study presents a relatively simple and reliable way to identify each axolotl LBC cytologically and to anchor chromosome-length sequences (from the axolotl genome assembly) to the physical LBCs by immunostaining and fluorescence in situ hybridization. Our data will facilitate a more detailed transcription analysis of individual LBC loops.

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