Benjamin W. Roose scite author profile

Molecular imaging holds considerable promise for elucidating biological processes in normal physiology as well as disease states, but requires noninvasive methods for identifying analytes at sub-micromolar concentrations. Particularly useful are genetically encoded, single-protein reporters that harness the power of molecular biology to visualize specific molecular processes, but such reporters have been conspicuously lacking for in vivo magnetic resonance imaging (MRI). Here, we report TEM-1 β-lactamase (bla) as a single-protein reporter for hyperpolarized (HP) 129Xe NMR, with significant saturation contrast at 0.1 μM. Xenon chemical exchange saturation transfer (CEST) interactions with the primary allosteric site in bla give rise to a unique saturation peak at 255 ppm, well removed (~60 ppm downfield) from the 129Xe-H2O peak. Useful saturation contrast was also observed for bla expressed in bacterial cells and mammalian cells.

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Cryptophane Nanoscale Assemblies Expand ¹²⁹Xe NMR Biosensing

Zemerov

Roose

Greenberg

et al. 2018

Anal. Chem.

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Cryptophane-based biosensors are promising agents for the ultrasensitive detection of biomedically relevant targets via Xe NMR. Dynamic light scattering revealed that cryptophanes form water-soluble aggregates tens to hundreds of nanometers in size. Acridine orange fluorescence quenching assays allowed quantitation of the aggregation state, with critical concentrations ranging from 200 nM to 600 nM, depending on the cryptophane species in solution. The addition of excess carbonic anhydrase (CA) protein target to a benzenesulfonamide-functionalized cryptophane biosensor (C8B) led to C8B disaggregation and produced the expected 1:1 C8B-CA complex. C8B showed higher affinity at 298 K for the cytoplasmic isozyme CAII than the extracellular CAXII isozyme, which is a biomarker of cancer. Using hyper-CEST NMR, we explored the role of stoichiometry in detecting these two isozymes. Under CA-saturating conditions, we observed that isozyme CAII produces a largerXe NMR chemical shift change (δ = 5.9 ppm, relative to free biosensor) than CAXII (δ = 2.7 ppm), which indicates the strong potential for isozyme-specific detection. However, stoichiometry-dependent chemical shift data indicated that biosensor disaggregation contributes to the observed Xe NMR chemical shift change that is normally assigned to biosensor-target binding. Finally, we determined that monomeric cryptophane solutions improve hyper-CEST saturation contrast, which enables ultrasensitive detection of biosensor-protein complexes. These insights into cryptophane-solution behavior support further development of xenon biosensors, but will require reinterpretation of the data previously obtained for many water-soluble cryptophanes.

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Thermophilic Ferritin 24mer Assembly and Nanoparticle Encapsulation Modulated by Interdimer Electrostatic Repulsion

et al. 2017

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Protein cage self-assembly enables encapsulation and sequestration of small molecules, macromolecules, and nanomaterials for many applications in bionanotechnology. Notably, wild-type thermophilic ferritin from Archaeoglobus fulgidus (AfFtn) exists as a stable dimer of four-helix bundle proteins at low ionic strength, and the protein forms a hollow assembly of 24 protomers at high ionic strength (∼800 mM NaCl). This assembly process can also be initiated by highly charged gold nanoparticles (AuNPs) in solution, leading to encapsulation. These data suggest that salt solutions or charged AuNPs can shield unfavorable electrostatic interactions at AfFtn dimer-dimer interfaces, but specific “hot-spot” residues controlling assembly have not been identified. To investigate this further, we computationally designed three AfFtn mutants (E65R, D138K, A127R) that introduce a single positive charge at sites along the dimer-dimer interface. These proteins exhibited different assembly kinetics and thermodynamics, which were ranked in order of increasing 24mer propensity: A127R < WT < D138K ≪ E65R. E65R assembled to the 24mer across a wide range of ionic strengths (0 – 800 mM NaCl), and the dissociation temperature for the 24mer was 98 °C. X-ray crystal structure analysis of the E65R mutant identified a more compact, closed-pore cage geometry. A127R and D138K mutants exhibited wild-type ability to encapsulate and stabilize 5-nm AuNPs, whereas E65R gained ability to remain assembled in apo-form. This work illustrates designed protein cages with distinct assembly and encapsulation properties.

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Nanomolar small-molecule detection using a genetically encoded¹²⁹Xe NMR contrast agent

2017

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Benjamin W. Roose

A Genetically Encoded β‐Lactamase Reporter for Ultrasensitive ¹²⁹Xe NMR in Mammalian Cells

Cryptophane Nanoscale Assemblies Expand ¹²⁹Xe NMR Biosensing

Thermophilic Ferritin 24mer Assembly and Nanoparticle Encapsulation Modulated by Interdimer Electrostatic Repulsion

Nanomolar small-molecule detection using a genetically encoded¹²⁹Xe NMR contrast agent

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Benjamin W. Roose

A Genetically Encoded β‐Lactamase Reporter for Ultrasensitive 129Xe NMR in Mammalian Cells

Cryptophane Nanoscale Assemblies Expand 129Xe NMR Biosensing

Thermophilic Ferritin 24mer Assembly and Nanoparticle Encapsulation Modulated by Interdimer Electrostatic Repulsion

Nanomolar small-molecule detection using a genetically encoded129Xe NMR contrast agent

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Product

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A Genetically Encoded β‐Lactamase Reporter for Ultrasensitive ¹²⁹Xe NMR in Mammalian Cells

Cryptophane Nanoscale Assemblies Expand ¹²⁹Xe NMR Biosensing

Nanomolar small-molecule detection using a genetically encoded¹²⁹Xe NMR contrast agent