Publications by authors named "Loic Lindner"

Copy number variations (CNVs) of the human 16p11.2 locus are associated with several developmental/neurocognitive syndromes. Particularly, deletion and duplication of this genetic interval are found in patients with autism spectrum disorders, intellectual disability and other psychiatric traits.

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Background: Animal models are essential to understand the physiopathology of human diseases but also to evaluate new therapies. However, for several diseases there is no appropriate animal model, which complicates the development of effective therapies. HPV infections, responsible for carcinoma cancers, are among these.

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CRISPR/Cas9 technology is a versatile tool for engineering biology that has dramatically transformed our ability to manipulate genomes. In this protocol, we use its capacity to generate two double-strand breaks simultaneously, at precise positions in the genome, to generate mouse or rat lines with deletion, inversion, and duplication of a specific genomic segment. The technic is called CRISMERE for CRISpr-MEdiated REarrangement.

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The French mouse clinic (Institut Clinique de la Souris; ICS) has produced more than 2000 targeting vectors for 'à la carte' mutagenesis in C57BL/6N mice. Although most of the vectors were used successfully for homologous recombination in murine embryonic stem cells (ESCs), a few have failed to target a specific locus after several attempts. We show here that co-electroporation of a CRISPR plasmid with the same targeting construct as the one that failed previously allows the systematic achievement of positive clones.

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Article Synopsis
  • Perturbation of the excitation/inhibition (E/I) balance is linked to neurodevelopmental disorders like autism, intellectual disability, and epilepsy, with mutations in the DYRK1A gene on chromosome 21 being a significant factor.
  • Research using a specific mouse model examined the effects of varying copies of the Dyrk1a gene in glutamatergic neurons, revealing its crucial role in long-term explicit memory without affecting locomotor activity or seizure risk.
  • Findings include that DYRK1A influences transcriptional activity and interacts with post-synaptic proteins, providing insights that could inform future therapeutic strategies targeting DYRK1A inhibitors.
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Gene targeting and additive (random) transgenesis have proven to be powerful technologies with which to decipher the mammalian genome. With the advent of CRISPR/Cas9 genome editing, the ability to inactivate or modify the function of a gene has become even more accessible. However, the impact of each generated modification may be different from what was initially desired.

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Droplet digital PCR (ddPCR) is a recent method developed for the quantification of nucleic acids sequences. It is an evolution of PCR methodology incorporating two principal differences: a PCR reaction is performed in thousands of water-oil emulsion droplets and fluorescence is measured at the end of PCR amplification. It leads to the precise and reproducible quantification of DNA and RNA sequences.

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Article Synopsis
  • ATP6AP2 is a gene that helps make a receptor important for converting a substance in the body, which is why it's a target for new drugs.
  • When scientists turned off this gene in mice, it caused serious problems in different organs, showing it's really important for health.
  • If ATP6AP2 is disrupted in adult mice, they quickly get sick and even die, highlighting that any drugs affecting this gene must be very carefully tested to avoid harm.
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Modelling Down syndrome (DS) in mouse has been crucial for the understanding of the disease and the evaluation of therapeutic targets. Nevertheless, the modelling so far has been limited to the mouse and, even in this model, generating duplication of genomic regions has been labour intensive and time consuming. We developed the CRISpr MEdiated REarrangement (CRISMERE) strategy, which takes advantage of the CRISPR/Cas9 system, to generate most of the desired rearrangements from a single experiment at much lower expenses and in less than 9 months.

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Article Synopsis
  • Scientists studied mouse cells to make sure they were healthy for future generations.
  • They found that if too many cells have chromosome problems, it makes it harder for them to successfully pass on their genes.
  • A new method using special tests helped them quickly check the cells for issues, so they could avoid using the ones that might not work well.
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