Targeted Bioimaging of Microencapsulated Recombinant LAB Vector Expressing Fluorescent Reporter Protein: A Non-invasive Approach for Microbial Tracking.

IF 5.4 2区 医学 Q2 MATERIALS SCIENCE, BIOMATERIALS ACS Biomaterials Science & Engineering Pub Date : 2024-08-12 Epub Date: 2024-08-01 DOI:10.1021/acsbiomaterials.4c00597
Prakash Biswas, Afruja Khan, Amirul Islam Mallick
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Abstract

Lactococcus lactis (L. lactis), the first genetically modified Generally Recognized As Safe (GRAS) category Lactic Acid producing Bacteria (LAB), is best known for its generalized health-promoting benefits and ability to express heterologous proteins. However, achieving the optimal probiotic effects requires a selective approach that would allow us to study in vivo microbial biodistribution, fate, and immunological consequences. Although the chemical conjugation of fluorophores and chromophores represent the standard procedure to tag microbial cells for various downstream applications, it requires a high-throughput synthesis scheme, which is often time-consuming and expensive. On the contrary, the genetic manipulation of LAB vector, either chromosomally or extra-chromosomally, to express bioluminescent or fluorescent reporter proteins has greatly enhanced our ability to monitor bacterial transit through a complex gut environment. However, with faster passage and quick washing out from the gut due to rhythmic contractions of the digestive tract, real-time tracking of LAB vectors, particularly non-commensal ones, remains problematic. To get a deeper insight into the biodistribution of non-commensal probiotic bacteria in vivo, we bioengineered L. lactis to express fluorescence reporter proteins, mCherry (bright red monomeric fluorescent protein) and mEGFP (monomeric enhanced green fluorescent protein), followed by microencapsulation with a mucoadhesive and biodegradable polymer, chitosan. We show that coating of recombinant Lactococcus lactis (rL. lactis) with chitosan polymer, cross-linked with tripolyphosphate (TPP), retains their ability to express the reporter proteins stably without altering the specificity and sensitivity of fluorescence detection in vitro and in vivo. Further, we provide evidence of enhanced intragastric stability by chitosan-TPP (CS) coating of rL. lactis cells, allowing us to study the spatiotemporal distribution for an extended time in the gut of two unrelated hosts, avian and murine. The present scheme involving genetic modification and chitosan encapsulation of non-commensal LAB vector demonstrates great promise as a non-invasive and intensive tool for active live tracking of gut microbes.

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表达荧光报告蛋白的微囊重组 LAB 载体的靶向生物成像:微生物追踪的非侵入性方法。
乳酸乳球菌(Lactococcus lactis,简称 L.lactis)是第一种转基因的公认安全(GRAS)类乳酸菌(LAB),因其促进健康的普遍益处和表达异源蛋白的能力而闻名于世。然而,要达到最佳的益生菌效果,需要一种选择性方法,使我们能够研究体内微生物的生物分布、转归和免疫后果。虽然荧光团和发色团的化学共轭是标记微生物细胞以用于各种下游应用的标准程序,但它需要高通量的合成方案,通常既耗时又昂贵。相反,通过对 LAB 载体进行染色体或染色体外的遗传操作来表达生物发光或荧光报告蛋白,大大提高了我们监测细菌在复杂肠道环境中转运的能力。然而,由于消化道的节律性收缩导致细菌通过肠道的速度加快,并很快被冲出肠道,因此对 LAB 载体(尤其是非共生载体)的实时跟踪仍然存在问题。为了更深入地了解非共生益生菌在体内的生物分布情况,我们对乳酸杆菌进行了生物工程改造,使其表达荧光报告蛋白 mCherry(鲜红色单体荧光蛋白)和 mEGFP(单体增强型绿色荧光蛋白),然后用粘液粘附性和生物可降解聚合物壳聚糖进行微囊化。我们的研究表明,用三聚磷酸钠(TPP)交联的壳聚糖聚合物包覆重组乳球菌(rL. lactis),可保持其稳定表达报告蛋白的能力,而不会改变体外和体内荧光检测的特异性和灵敏度。此外,我们还提供了通过壳聚糖-TPP(CS)包被 rL. lactis 细胞来增强其胃内稳定性的证据,从而使我们能够研究其在禽类和鼠类这两种不相关宿主肠道中长期的时空分布情况。本方案涉及非同源 LAB 载体的基因修饰和壳聚糖封装,作为一种非侵入性和密集型工具,它在主动活体追踪肠道微生物方面大有可为。
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来源期刊
ACS Biomaterials Science & Engineering
ACS Biomaterials Science & Engineering Materials Science-Biomaterials
CiteScore
10.30
自引率
3.40%
发文量
413
期刊介绍: ACS Biomaterials Science & Engineering is the leading journal in the field of biomaterials, serving as an international forum for publishing cutting-edge research and innovative ideas on a broad range of topics: Applications and Health – implantable tissues and devices, prosthesis, health risks, toxicology Bio-interactions and Bio-compatibility – material-biology interactions, chemical/morphological/structural communication, mechanobiology, signaling and biological responses, immuno-engineering, calcification, coatings, corrosion and degradation of biomaterials and devices, biophysical regulation of cell functions Characterization, Synthesis, and Modification – new biomaterials, bioinspired and biomimetic approaches to biomaterials, exploiting structural hierarchy and architectural control, combinatorial strategies for biomaterials discovery, genetic biomaterials design, synthetic biology, new composite systems, bionics, polymer synthesis Controlled Release and Delivery Systems – biomaterial-based drug and gene delivery, bio-responsive delivery of regulatory molecules, pharmaceutical engineering Healthcare Advances – clinical translation, regulatory issues, patient safety, emerging trends Imaging and Diagnostics – imaging agents and probes, theranostics, biosensors, monitoring Manufacturing and Technology – 3D printing, inks, organ-on-a-chip, bioreactor/perfusion systems, microdevices, BioMEMS, optics and electronics interfaces with biomaterials, systems integration Modeling and Informatics Tools – scaling methods to guide biomaterial design, predictive algorithms for structure-function, biomechanics, integrating bioinformatics with biomaterials discovery, metabolomics in the context of biomaterials Tissue Engineering and Regenerative Medicine – basic and applied studies, cell therapies, scaffolds, vascularization, bioartificial organs, transplantation and functionality, cellular agriculture
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