Masahiro Takinoue

Rapid Detection of a Cocaine-Binding Aptamer Using Biological Nanopores on a Chip

This paper describes a methodology for the rapid and highly selective detection of cocaine using a membrane protein channel combined with a DNA aptamer. The DNA aptamer recognizes the cocaine molecule with high selectivity. We successfully detected a low concentration of cocaine (300 ng/mL, the drug test cutoff limit) within 60 s using a biological nanopore embedded in a microchip.

Controlled Synthesis of 3D Multi‐Compartmental Particles with Centrifuge‐Based Microdroplet Formation from a Multi‐Barrelled Capillary

Controlled synthesis of micro multi-compartmental particles using a centrifuge droplet shooting device (CDSD) is reported. Sodium alginate solutions introduced in a multi-barreled capillary form droplets at the capillary orifice under ultrahigh gravity and gelify in a CaCl(2) solution. The size, shape, and compartmentalization of the particles are controlled. Co-encapsulation of Jurkat cells and magnetic colloids into Janus particles is demonstrated. The Janus particles present sensitive reaction toward magnetic fields, while the viability of the encapsulated cells is 91%.

Feedback control of protein expression in mammalian cells by tunable synthetic translational inhibition.

Feedback regulation plays a crucial role in dynamic gene expression in nature, but synthetic translational feedback systems have yet to be demonstrated. Here we use an RNA/protein interaction-based synthetic translational switch to create a feedback system that tightly controls the expression of proteins of interest in mammalian cells. Feedback is mediated by modified ribosomal L7Ae proteins, which bind a set of RNA motifs with a range of affinities. We designed these motifs into L7Ae-encoding mRNA. Newly translated L7Ae binds its own mRNA, inhibiting further translation. This inhibition tightly feedback-regulates the concentration of L7Ae and any fusion partner of interest. A mathematical model predicts system behavior as a function of RNA/protein affinity. We further demonstrate that the L7Ae protein can simultaneously and tunably regulate the expression of multiple proteins of interest by binding RNA control motifs built into each mRNA, allowing control over the coordinated expression of protein networks.

Droplet microfluidics for the study of artificial cells.

In this review, we describe recent advances in droplet-based microfluidics technology that can be applied in studies of artificial cells. Artificial cells are simplified models of living cells and provide valuable model platforms designed to reveal the functions of biological systems. The study of artificial cells is promoted by microfluidics technologies, which provide control over tiny volumes of solutions during quantitative chemical experiments and other manipulations. Here, we focus on current and future trends in droplet microfluidics and their applications in studies of artificial cells.

Rotary motion driven by a direct current electric field

We report the rotary motion of an aqueous microdroplet in an oil phase under a stationary direct current electric field. A droplet exhibits rotary motion under a suitable geometrical arrangement of positive and negative electrodes. Rotary motion appears above a certain critical electric potential and its frequency increases with an increase in the potential. A simple theoretical model is proposed to describe the occurrence of this rotary motion, together with an argument for the future expansion of this micro rotary motor system.

Tunable synthetic phenotypic diversification on Waddington’s landscape through autonomous signaling

Phenotypic diversification of cells is crucial for developmental and regenerative processes in multicellular organisms. The diversification concept is described as the motion of marbles rolling down Waddington’s landscape, in which the number of stable states changes as development proceeds. In contrast to this simple concept, the complexity of natural biomolecular processes prevents comprehension of their design principles. We have constructed, in Escherichia coli, a synthetic circuit with just four genes, which programs cells to autonomously diversify as the motion on the landscape through cell–cell communication. The circuit design was based on the combination of a bistable toggle switch with an intercellular signaling system. The cells with the circuit diversified into two distinct cell states, “high” and “low,” in vivo and in silico, when all of the cells started from the low state. The synthetic diversification was affected by not only the shape of the landscape determined by the circuit design, which includes the synthesis rate of the signaling molecule, but also the number of cells in the experiments. This cell-number dependency is reminiscent of the “community effect”: The fates of developing cells are determined by their number. Our synthetic circuit could be a model system for studying diversification and differentiation in higher organisms. Prospectively, further integrations of our circuit with different cellular functions will provide unique tools for directing cell fates on the population level in tissue engineering.

RTRACS: a modularized RNA-dependent RNA transcription system with high programmability.

Creating artificial biological systems is an important research endeavor. Each success contributes to synthetic biology and adds to our understanding of the functioning of the biomachinery of life. In the construction of large, complex systems, a modular approach simplifies the design process: a multilayered system can be prepared by integrating simple modules. With the concept of modularity, a variety of synthetic biological systems have been constructed, both in vivo and in vitro. But to properly develop systems with desired functions that integrate multiple modules, researchers need accurate mathematical models. In this Account, we review the development of a modularized artificial biological system known as RTRACS (reverse transcription and transcription-based autonomous computing system). In addition to modularity, model-guided predictability is an important feature of RTRACS. RTRACS has been developed as an in vitro artificial biological system through the assembly of RNA, DNA, and enzymes. A fundamental module of RTRACS receives an input RNA with a specific sequence and returns an output RNA with another specific sequence programmed in the main body, which is composed of DNA and enzymes. The conversion of the input RNA to the output RNA is achieved through a series of programmed reactions performed by the components assembled in the module. Through the substitution of a subset of components, a module that performs the AND operation was constructed. Other logical operations could be constructed with RTRACS modules. An integration of RTRACS modules has allowed the theoretical design of more complex functions, such as oscillation. The operations of these RTRACS modules were readily predicted with a numerical simulation based on a mathematical model using realistic parameters. RTRACS has the potential to model highly complex systems that function like a living cell. RTRACS was designed to be integrated with other molecules or molecular devices, for example, aptazymes, cell-free expression systems, and liposomes. For the integration of these new modules, the quantitative controls of each module based on the numerical simulation will be instructive. The capabilities of RTRACS promise to provide models of complex biomolecular systems that are able to detect the environment, assess the situation, and react to overcome the situation. Such a smart biomolecular system could be useful in many applications, such as drug delivery systems.

Complex-shaped three-dimensional multi-compartmental microparticles generated by diffusional and Marangoni microflows in centrifugally discharged droplets

We report a versatile method for the generation of complex-shaped three-dimensional multi-compartmental (3D-MC) microparticles. Complex-shaped microparticles have recently received much attention for potential application in self-assemblies, micromachines, and biomedical and environmental engineering. Here, we have developed a method based on 3D nonequilibrium-induced microflows (Marangoni and diffusional flows) of microdroplets that are discharged from the tip of a thin capillary in a simple centrifugal microfluidic device. The microparticle shapes can be tuned by the partial dissolution of specific compartments and by the deformation of the precursor microdroplets by manipulating the 3D microflows. We believe that this method will have wide applications in nano- and microscience and technologies.

Centrifuge-based cell encapsulation in hydrogel microbeads using sub-microliter sample solution

This paper describes a simple, rapid, and inexpensive method for cell encapsulation that uses a small amount (sub-microliter-scale) of cell-suspended pre-gel solution. This method requires only a glass capillary, an acrylic holder, and a tabletop centrifuge, and achieves cell encapsulation in calcium alginate microbeads using cell-suspended sub-microliter-volume pre-gel solution in 20 s. The method also ensures high cell encapsulation efficiency, with a sample loss of as low as several tens of nanoliters. Formation of calcium alginate hydrogel microbeads encapsulating Jurkat cells by the proposed method is experimentally demonstrated using 0.5 μL of cell-suspended sodium alginate solution. Our proposed method is expected to be a promising approach for encapsulating rare and precious samples by non-specialists of microfluidics working in the fields of point-of-care and tailor-made medicine.

DNA cytoskeleton for stabilizing artificial cells

Significance Although liposomes and lipid droplets have been used for numerous applications, the fragility of the lipid membrane causes an unintentional collapse, which is problematic for advanced applications. To solve this problem, we constructed an artificial cytoskeleton with DNA nanotechnology (a DNA cytoskeleton). The DNA cytoskeleton is a DNA network formed underneath the membrane of positively charged lipids through electrostatic interactions without the need for special handling. The DNA cytoskeleton significantly improves mechanical stability and, therefore, confers tolerance against osmotic shock to liposomes like the cytoskeleton in live cells. Because of its biocompatibility and the easiness of implementing design changes, the DNA cytoskeleton could become a tool for great stabilizer of liposomes and lipid droplets. Cell-sized liposomes and droplets coated with lipid layers have been used as platforms for understanding live cells, constructing artificial cells, and implementing functional biomedical tools such as biosensing platforms and drug delivery systems. However, these systems are very fragile, which results from the absence of cytoskeletons in these systems. Here, we construct an artificial cytoskeleton using DNA nanostructures. The designed DNA oligomers form a Y-shaped nanostructure and connect to each other with their complementary sticky ends to form networks. To undercoat lipid membranes with this DNA network, we used cationic lipids that attract negatively charged DNA. By encapsulating the DNA into the droplets, we successfully created a DNA shell underneath the membrane. The DNA shells increased interfacial tension, elastic modulus, and shear modulus of the droplet surface, consequently stabilizing the lipid droplets. Such drastic changes in stability were detected only when the DNA shell was in the gel phase. Furthermore, we demonstrate that liposomes with the DNA gel shell are substantially tolerant against outer osmotic shock. These results clearly show the DNA gel shell is a stabilizer of the lipid membrane akin to the cytoskeleton in live cells.