Single-molecule
localization microscopy (SMLM) enables the visualization
of biomolecules at unprecedented resolution and requires control of
the fluorescent blinking (ON/OFF) states of fluorophores to detect
single-molecule fluorescence without overlapping of the signals. Although
SMLM probes based on the intramolecular spirocyclization of Si-xanthene
fluorophores have been developed, fluorophores with lower ON/OFF ratios
are required for SMLM visualization of high-density structures. Here,
we describe a silinane structure that lowers the ON/OFF ratio of Si-xanthene
fluorophores. On the basis of Mulliken population analysis, we replaced
the dimethylsilane moiety in Si-rhodamine with a silinane moiety to
increase the partial charge at the 9-position of the carbon atom in
the Si-xanthene ring and to promote the ring-closure reaction. Evaluation
of fluorescence properties in a solution and in single-molecule imaging
indicated that introducing the silinane sufficiently stabilized the
nonfluorescent spirocyclic forms, thus decreasing the fluorescence
ON/OFF ratio. This novel substitution was applied to Si-rhodamines
with various amine structures and to an Si-fluorescein to expand the
color palette. We demonstrated SMLM observation of microtubules in
fixed HeLa cells using the developed fluorophores in two color channels.
The results demonstrated the feasibility of extending the design strategies
of SMLM probes based on Si-xanthenes through modification of the substituents
on the Si atom.
Process development of E2609 from the preclinical stage to the clinical stage following a process risk mitigation strategy is described here. Key features include a turbo Grignard reaction monitored by in-situ IR, [3 + 2] cycloaddition in water, chemoselective amide coupling via in-situ protection, and a Reformatsky/decarboxylation approach to install a difluoromethyl group. Toward safe and scalable manufacture of E2071, an analog of E2609, a flow-reaction process for trifluoromethylation of aldehydes is presented here.
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