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  2. Frequency-Selective Microbubble Targeting In Vitro: A Step Toward Multicolor Ultrasound Molecular Imaging

Frequency-Selective Microbubble Targeting In Vitro: A Step Toward Multicolor Ultrasound Molecular Imaging

  • ACS Appl Bio Mater. 2025 Mar 17;8(3):2128-2140. doi: 10.1021/acsabm.4c01699.
Jair I Castillo 1 J Angel Navarro-Becerra 2 Ilaria Angelini 1 3 Maxim Kokoshinskiy 1 Mark A Borden 1 2
Affiliations

Affiliations

  • 1 Biomedical Engineering Program, University of Colorado, Boulder, Colorado 80309, United States.
  • 2 Mechanical Engineering Department, University of Colorado, Boulder, Colorado 80309, United States.
  • 3 Chemistry Department, University of Rome Tor Vergata, Rome 00133, Italy.
Abstract

Ultrasound molecular imaging (USMI) utilizing targeted microbubbles (tMBs) and primary acoustic radiation force (Frad) pulses has demonstrated enhanced sensitivity in recent studies. However, current USMI techniques are limited to a single ligand-receptor pair per imaging scan. With the advent of the buried-ligand architecture (BLA), "cloaked" ligand-receptor binding and tMB adhesion can be activated by Frad pulses, enabling multicolor USMI. This approach permits the selective activation of two or more tMB species, each binding to its cognate receptors based on distinct resonance frequencies (f0) tuned by Frad pulses. The goal of this study was to demonstrate frequency-selective tMB adhesion to receptor-bearing microvessel tubes in vitro. Size-isolated BLA tMBs of 1 and 5 μm diameter were synthesized with f0 equal to 7 and 4 MHz, respectively (within the frequency limits of our ultrasound probe). The 1 μm tMBs were conjugated with IELLQAR peptide for P-selectin targeting, while the 5 μm tMBs were conjugated with cyclo-RGD peptide for αvβ3 Integrin targeting. The MB gas volume fraction (φMB) was used to unify size and concentration into a single parameter. Frequency-selective tMB binding was quantified using fluorescence microscopy. Specific targeting was evaluated by comparing RGD- or IELLQAR-MB attachment to control RAD- or nonligand-bearing MBs, respectively. The results confirmed specific frequency-selective targeting of the two tMB species to their cognate receptors when activated by Frad pulses at their respective f0, both individually and in a cocktail. In the cocktail population, φMB of RGD-MB targeting increased 18-fold at 4 MHz compared to 7 MHz, while IELLQAR-MB targeting φMB increased 5-fold at 7 MHz compared to 4 MHz. In conclusion, this study presents the first demonstration of frequency-selective targeting of two different receptor species by two different tMB species, representing a significant step toward multicolor USMI and the potential for simultaneous imaging of multiple biomarkers in vivo within a single scan.

Keywords

buried-ligand architecture; ligand receptor specificity; primary radiation force; resonance frequency; size-isolated microbubbles.

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