4.2 Article

A cryo-fixation protocol to study the structure of the synaptonemal complex

Journal

CHROMOSOME RESEARCH
Volume 30, Issue 4, Pages 385-400

Publisher

SPRINGER
DOI: 10.1007/s10577-022-09689-2

Keywords

Synaptonemal complex; Meiosis; Cryo-fixation; Close-to-native structure

Funding

  1. Swedish Research Council [2017-01853]
  2. Hospital Infantil de Mexico Federico Gomez [HIM/2018/079 SSA 1518, HIM/2021/061]
  3. Swedish Research Council [2017-01853] Funding Source: Swedish Research Council

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This study analyzed the structure of the synaptonemal complex (SC) using cryo-fixation and electron microscopy. Compared to chemical fixation, cryo-fixation showed differences in the width of the central region of the SC and the density of the transverse filaments.
Genetic variability in sexually reproducing organisms results from an exchange of genetic material between homologous chromosomes. The genetic exchange mechanism is dependent on the synaptonemal complex (SC), a protein structure localized between the homologous chromosomes. The current structural models of the mammalian SC are based on electron microscopy, superresolution, and expansion microscopy studies using chemical fixatives and sample dehydration of gonads, which are methodologies known to produce structural artifacts. To further analyze the structure of the SC, without chemical fixation, we have adapted a cryo-fixation method for electron microscopy where pachytene cells are isolated from mouse testis by FACS, followed by cryo-fixation, cryo-substitution, and electron tomography. In parallel, we performed conventional chemical fixation and electron tomography on mouse seminiferous tubules to compare the SC structure obtained with the two fixation methods. We found several differences in the structure and organization of the SC in cryo-fixed samples when compared to chemically preserved samples. We found the central region of the SC to be wider and the transverse filaments to be more densely packed in the central region of the SC.

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