Abstract

Principles of molecular self-assembly into giant hierarchical structures of hundreds of micrometers in size are studied in aggregates of meso-tetra(4-sulfonatophenyl)porphine (TPPS4). The aggregates form a central tubular core, which is covered with radially protruding filamentous non-branching aggregates. The filaments cluster and orient at varying angles from the core surface and some filaments form bundles. Due to shape resemblance, the structures are termed giant sea urchin (GSU) aggregates. Spectrally resolved fluorescence microscopy reveals J- and H-bands of TPPS4 aggregates in both the central core and the filaments. The fluorescence of the core is quenched while filaments exhibit strong fluorescence. Upon drying, the filament fluorescence gets quenched while the core is less affected, showing stronger relative fluorescence. Fluorescence-detected linear dichroism (FDLD) microscopy reveals that absorption dipoles corresponding to J-bands are oriented along the filament axis. The comparison of FDLD with scanning electron microscopy (SEM) reveals the structure of central core comprised of multilayer ribbons, which wind around the core axis forming a tube. Polarimetric second-harmonic generation (SHG) and third-harmonic generation microscopy exhibits strong signal from the filaments with nonlinear dipoles oriented close to the filament axis, while central core displays very low SHG due to close to centrosymmetric organization. Large chiral nonlinear susceptibility points to helical arrangement of the filaments. The investigation shows that TPPS4 molecules form distinct aggregate types, including chiral nanotubes and nanogranular aggregates that associate into the hierarchical GSU structure, prototypical to complex biological structures. The chiral TPPS4 aggregates can serve as harmonophores for nonlinear microscopy.

Highlights

  • Principles of molecular self-assembly into giant hierarchical structures of hundreds of micrometers in size are studied in aggregates of meso-tetra(4-sulfonatophenyl)porphine (TPPS4)

  • Fluorescencedetected linear dichroism (FDLD) microscopy reveals that absorption dipoles corresponding to J-bands are oriented along the filament axis

  • The comparison of FDLD with scanning electron microscopy (SEM) reveals the structure of central core comprised of multilayer ribbons, which wind around the core axis forming a tube

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Summary

Materials

5114 XBT QVSDIBTFE GSPN 4JHNB "MESJDI 4U -PVJT .JTTPVSJ 64" BOE VTFE XJUIPVU GVSUIFS QVSJGJDBUJPO 'PS TBNQMF JNNPCJMJ[BUJPO UIF

Brightfield and spectral confocal fluorescence microscopy
Fluorescence-detected linear dichroism microscopy
Multimodal second- and third-harmonic generation microscopy
Laser scanning confocal and spectrally resolved fluorescence microscopy
Fluorescence-detected polarization microscopy
Correlation between SEM and FDLD microscopy data
Second- and third-harmonic generation microscopy
Structure and self-assembly of the GSU aggregate 5IF DFOUSBM DPSF BOE UIF GJMBNFOUT PG B (46 BHHSFHBUF TFMG
Structure of the filaments
Varying attachment angle of the filament clusters to the core surface
Energy transfer in GSU aggregates

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