Your search keyword '"Peñate-Medina T"' showing total 10 results

1. Gut microbiome-derived bacterial extracellular vesicles in patients with solid tumours

Author

Mishra, Surbhi, Tejesvi, Mysore Vishakantegowda, Hekkala, Jenni, Turunen, Jenni, Kandikanti, Niyati, Kaisanlahti, Anna, Suokas, Marko, Leppä, Sirpa, Vihinen, Pia, Kuitunen, Hanne, Sunela, Kaisa, Koivunen, Jussi, Jukkola, Arja, Kalashnikov, Ilja, Auvinen, Päivi, Kääriäinen, Okko-Sakari, Peñate Medina, T., Peñate Medina, O., Saarnio, Juha, Meriläinen, Sanna, Rautio, Tero, Aro, Raila, Häivälä, Reetta, Suojanen, Juho, Laine, Mikael, Erawijattari, Pande Putu, Lahti, Leo, Karihtala, Peeter, Ruuska, Terhi S., and Reunanen, Justus

Published

2025

2. Photoakustik für die präklinische skelettale Bildgebung

Author

Humbert, J, additional, Will, O, additional, Peñate Medina, T, additional, Peñate Medina, O, additional, Glüer, C, additional, Jansen, O, additional, and Both, M, additional

Published

2019

3. Universal membrane-labeling combined with expression of Katushka far-red fluorescent protein enables non-invasive dynamic and longitudinal quantitative 3D dual-color fluorescent imaging of multiple bacterial strains in mouse intestine

Author

Peñate-Medina, O. (Oula), Tower, R. J. (Robert J.), Peñate-Medina, T. (Tuula), Will, O. (Olga), Saris, P. E. (Per E. J.), Suojanen, J. (Juho), Sorsa, T. (Timo), Huuskonen, L. (Laura), Hiippala, K. (Kaisa), Satokari, R. (Reetta), Glüer, C. C. (Claus C.), de Vos, W. M. (Willem M.), Reunanen, J. (Justus), Peñate-Medina, O. (Oula), Tower, R. J. (Robert J.), Peñate-Medina, T. (Tuula), Will, O. (Olga), Saris, P. E. (Per E. J.), Suojanen, J. (Juho), Sorsa, T. (Timo), Huuskonen, L. (Laura), Hiippala, K. (Kaisa), Satokari, R. (Reetta), Glüer, C. C. (Claus C.), de Vos, W. M. (Willem M.), and Reunanen, J. (Justus)

Abstract

Background: The human gastrointestinal (GI) tract microbiota has been a subject of intense research throughout the 3rd Millennium. Now that a general picture about microbiota composition in health and disease is emerging, questions about factors determining development of microbiotas with specific community structures will be addressed. To this end, usage of murine models for colonization studies remains crucial. Optical in vivo imaging of either bioluminescent or fluorescent bacteria is the basis for non-invasive detection of intestinal colonization of bacteria. Although recent advances in in vivo fluorescence imaging have overcome many limitations encountered in bioluminescent imaging of intestinal bacteria, such as requirement for live cells, high signal attenuation and 2D imaging, the method is still restricted to bacteria for which molecular cloning tools are available. Results: Here, we present usage of a lipophilic fluorescent dye together with Katushka far-red fluorescent protein to establish a dual-color in vivo imaging system to monitor GI transit of different bacterial strains, suitable also for strains resistant to genetic labeling. Using this system, we were able to distinguish two different E. coli strains simultaneously and show their unique transit patterns. Combined with fluorescence molecular tomography, these distinct strains could be spatially and temporally resolved and quantified in 3D. Conclusions: Developed novel method for labeling microbes and identify their passage both temporally and spatially in vivo makes now possible to monitor all culturable bacterial strains, also those that are resistant to conventional genetic labeling.

Published

2019

4. Imaging Inflammation - From Whole Body Imaging to Cellular Resolution.

Author

Peñate Medina T, Kolb JP, Hüttmann G, Huber R, Peñate Medina O, Ha L, Ulloa P, Larsen N, Ferrari A, Rafecas M, Ellrichmann M, Pravdivtseva MS, Anikeeva M, Humbert J, Both M, Hundt JE, and Hövener JB

Subjects

Animals, Diagnostic Imaging, Humans, Inflammation diagnostic imaging

Abstract

Imaging techniques have evolved impressively lately, allowing whole new concepts like multimodal imaging, personal medicine, theranostic therapies, and molecular imaging to increase general awareness of possiblities of imaging to medicine field. Here, we have collected the selected (3D) imaging modalities and evaluated the recent findings on preclinical and clinical inflammation imaging. The focus has been on the feasibility of imaging to aid in inflammation precision medicine, and the key challenges and opportunities of the imaging modalities are presented. Some examples of the current usage in clinics/close to clinics have been brought out as an example. This review evaluates the future prospects of the imaging technologies for clinical applications in precision medicine from the pre-clinical development point of view., Competing Interests: The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest., (Copyright © 2021 Peñate Medina, Kolb, Hüttmann, Huber, Peñate Medina, Ha, Ulloa, Larsen, Ferrari, Rafecas, Ellrichmann, Pravdivtseva, Anikeeva, Humbert, Both, Hundt and Hövener.)

Published

2021

5. Acid-Sphingomyelinase Triggered Fluorescently Labeled Sphingomyelin Containing Liposomes in Tumor Diagnosis after Radiation-Induced Stress.

Author

Heneweer C, Peñate Medina T, Tower R, Kalthoff H, Kolesnick R, Larson S, and Peñate Medina O

Subjects

Animals, Catalysis, Cell Line, Tumor, Disease Models, Animal, Enzyme Activation, Mice, Molecular Imaging, Neoplasms radiotherapy, Optical Imaging, Sphingomyelins chemistry, Staining and Labeling, Fluorescent Dyes chemistry, Liposomes chemistry, Neoplasms diagnosis, Neoplasms metabolism, Sphingomyelin Phosphodiesterase metabolism, Sphingomyelins metabolism, Stress, Physiological radiation effects

Abstract

In liposomal delivery, a big question is how to release the loaded material into the correct place. Here, we will test the targeting and release abilities of our sphingomyelin-consisting liposome. A change in release parameters can be observed when sphingomyelin-containing liposome is treated with sphingomyelinase enzyme. Sphingomyelinase is known to be endogenously released from the different cells in stress situations. We assume the effective enzyme treatment will weaken the liposome making it also leakier. To test the release abilities of the SM-liposome, we developed several fluorescence-based experiments. In in vitro studies, we used molecular quenching to study the sphingomyelinase enzyme-based release from the liposomes. We could show that the enzyme treatment releases loaded fluorescent markers from sphingomyelin-containing liposomes. Moreover, the release correlated with used enzymatic activities. We studied whether the stress-related enzyme expression is increased if the cells are treated with radiation as a stress inducer. It appeared that the radiation caused increased enzymatic activity. We studied our liposomes' biodistribution in the animal tumor model when the tumor was under radiation stress. Increased targeting of the fluorescent marker loaded to our liposomes could be found on the site of cancer. The liposomal targeting in vivo could be improved by radiation. Based on our studies, we propose sphingomyelin-containing liposomes can be used as a controlled release system sensitive to cell stress.

Published

2021

6. Lipid-Iron Nanoparticle with a Cell Stress Release Mechanism Combined with a Local Alternating Magnetic Field Enables Site-Activated Drug Release.

Author

Peñate Medina T, Gerle M, Humbert J, Chu H, Köpnick AL, Barkmann R, M Garamus V, Sanz B, Purcz N, Will O, Appold L, Damm T, Suojanen J, Arnold P, Lucius R, Willumeit-Römer R, Açil Y, Wiltfang J, Goya GF, Glüer CC, and Peñate Medina O

Abstract

Most available cancer chemotherapies are based on systemically administered small organic molecules, and only a tiny fraction of the drug reaches the disease site. The approach causes significant side effects and limits the outcome of the therapy. Targeted drug delivery provides an alternative to improve the situation. However, due to the poor release characteristics of the delivery systems, limitations remain. This report presents a new approach to address the challenges using two fundamentally different mechanisms to trigger the release from the liposomal carrier. We use an endogenous disease marker, an enzyme, combined with an externally applied magnetic field, to open the delivery system at the correct time only in the disease site. This site-activated release system is a novel two-switch nanomachine that can be regulated by a cell stress-induced enzyme at the cellular level and be remotely controlled using an applied magnetic field. We tested the concept using sphingomyelin-containing liposomes encapsulated with indocyanine green, fluorescent marker, or the anticancer drug cisplatin. We engineered the liposomes by adding paramagnetic beads to act as a receiver of outside magnetic energy. The developed multifunctional liposomes were characterized in vitro in leakage studies and cell internalization studies. The release system was further studied in vivo in imaging and therapy trials using a squamous cell carcinoma tumor in the mouse as a disease model. In vitro studies showed an increased release of loaded material when stress-related enzyme and magnetic field was applied to the carrier liposomes. The theranostic liposomes were found in tumors, and the improved therapeutic effect was shown in the survival studies.

Published

2020

7. Comparison of photoacoustic and fluorescence tomography for the in vivo imaging of ICG-labelled liposomes in the medullary cavity in mice.

Author

Humbert J, Will O, Peñate-Medina T, Peñate-Medina O, Jansen O, Both M, and Glüer CC

Abstract

Few reports quantitatively compare the performance of photoacoustic tomography (PAT) versus fluorescence molecular tomography (FMT) in vivo . We compared both modalities for the detection of signals from injected ICG liposomes in the tibial medullary space of 10 BALB/c mice in vivo and ex vivo . Signals significantly correlated between modalities (R² = 0.69) and within each modality in vivo versus ex vivo (PAT: R² = 0.70, FMT: R² = 0.76). Phantom studies showed that signals at 4 mm depth are detected down to 3.3 ng ICG by PAT and 33 ng by FMT, with a nominal spatial resolution below 0.5 mm in PAT and limited to 1 mm in FMT. Our study demonstrates comparable in vivo sensitivity, but superior ex vivo sensitivity and in vivo resolution for our ICG liposomes of the VevoLAZR versus the FMT2500. PAT provides a useful new tool for the high-resolution imaging of bone marrow signals, for example for monitoring drug delivery., Competing Interests: The authors declare that there are no conflicts of interest., (© 2020 Published by Elsevier GmbH.)

Published

2020

8. Utilizing ICG Spectroscopical Properties for Real-Time Nanoparticle Release Quantification In vitro and In vivo in Imaging Setups.

Author

Peñate-Medina T, Kraas E, Luo K, Humbert J, Zhu H, Mertens F, Gerle M, Rohwedder A, Damoah C, Will O, Acil Y, Kairemo K, Wiltfang J, Glüer CC, Scherließ R, Sebens S, and Peñate-Medina OP

Subjects

Animals, Liposomes, Mice, Optical Imaging, Spectrum Analysis, Indocyanine Green, Nanoparticles

Abstract

Background: Nanoparticle imaging and tracking the release of the loaded material from the nanoparticle system have attracted significant attention in recent years. If the release of the loaded molecules could be monitored reliably in vivo, it would speed up the development of drug delivery systems remarkably., Methods: Here, we test a system that uses indocyanine green (ICG) as a fluorescent agent for studying release kinetics in vitro and in vivo from the lipid iron nanoparticle delivery system. The ICG spectral properties like its concentration dependence, sensitivity and the fluctuation of the absorption and emission wavelengths can be utilized for gathering information about the change of the ICG surrounding., Results: We have found that the absorption, fluorescence, and photoacoustic spectra of ICG in lipid iron nanoparticles differ from the spectra of ICG in pure water and plasma. We followed the ICG containing liposomal nanoparticle uptake into squamous carcinoma cells (SCC) by fluorescence microscopy and the in vivo uptake into SCC tumors in an orthotopic xenograft nude mouse model under a surgical microscope., Conclusion: Absorption and emission properties of ICG in the different solvent environment, like in plasma and human serum albumin, differ from those in aqueous solution. Photoacoustic spectral imaging confirmed a peak shift towards longer wavelengths and an intensity increase of ICG when bound to the lipids. The SCC cells showed that the ICG containing liposomes bind to the cell surface but are not internalized in the SCC-9 cells after 60 minutes of incubation. We also showed here that ICG containing liposomal nanoparticles can be traced under a surgical camera in vivo in orthotopic SCC xenografts in mice., (Copyright© Bentham Science Publishers; For any queries, please email at epub@benthamscience.net.)

Published

2020

9. Alpha-MSH Targeted Liposomal Nanoparticle for Imaging in Inflammatory Bowel Disease (IBD).

Author

Peñate-Medina T, Damoah C, Benezra M, Will O, Kairemo K, Humbert J, Sebens S, and Peñate-Medina O

Subjects

Animals, Fluorescent Dyes chemistry, Mice, Tissue Distribution, Inflammatory Bowel Diseases diagnostic imaging, Liposomes, Nanoparticles, Receptor, Melanocortin, Type 1 chemistry, alpha-MSH chemistry

Abstract

Background: The purpose of our study was to find a novel targeted imaging and drug delivery vehicle for inflammatory bowel disease (IBD). IBD is a common and troublesome disease that still lacks effective therapy and imaging options. As an attempt to improve the disease treatment, we tested αMSH for the targeting of nanoliposomes to IBD sites. αMSH, an endogenous tridecapeptide, binds to the melanocortin-1 receptor (MC1-R) and has anti-inflammatory and immunomodulating effects. MC1-R is found on macrophages, neutrophils and the renal tubule system. We formulated and tested a liposomal nanoparticle involving αMSH in order to achieve a specific targeting to the inflamed intestines., Methods: NDP-αMSH peptide conjugated to Alexa Fluor™ 680 was linked to the liposomal membrane via NSuccinyl PE and additionally loaded into the lumen of the liposomes. Liposomes without the αMSH-conjugate and free NDP-αMSH were used as a control. The liposomes were also loaded with ICG to track them. The liposomes were tested in DSS treated mice, which had received DSS via drinking water order to develop a model IBD. Inflammation severity was assessed by the Disease Activity Index (DAI) score and ex vivo histological CD68 staining of samples taken from different parts of the intestine. The liposome targeting was analyzed by analyzing the ICG and ALEXA 680 fluorescence in the intestine compared to the biodistribution., Results: NPD-αMSH was successfully labeled with Alexa and retained its biological activity. Liposomes were identified in expected regions in the inflamed bowel regions and in the kidneys, where MC1-R is abundant. In vivo liposome targeting correlated with the macrophage concentration at the site of the inflammation supporting the active targeting of the liposomes through αMSH. The liposomal αMSH was well tolerated by animals., Conclusion: This study opens up the possibility to further develop an αMSH targeted theranostic delivery to different clinically relevant applications in IBD inflammation but also opens possibilities for use in other inflammations like lung inflammation in Covid 19., (Copyright© Bentham Science Publishers; For any queries, please email at epub@benthamscience.net.)

Published

2020

10. Universal membrane-labeling combined with expression of Katushka far-red fluorescent protein enables non-invasive dynamic and longitudinal quantitative 3D dual-color fluorescent imaging of multiple bacterial strains in mouse intestine.

Author

Peñate-Medina O, Tower RJ, Peñate-Medina T, Will O, Saris PEJ, Suojanen J, Sorsa T, Huuskonen L, Hiippala K, Satokari R, Glüer CC, de Vos WM, and Reunanen J

Subjects

Animals, Escherichia coli metabolism, Fluorescent Dyes metabolism, Gastrointestinal Microbiome, Intravital Microscopy methods, Luminescent Proteins metabolism, Membrane Lipids metabolism, Mice, Tomography, Optical, Red Fluorescent Protein, Gastrointestinal Tract microbiology, Microscopy, Fluorescence methods, Staining and Labeling methods

Abstract

Background: The human gastrointestinal (GI) tract microbiota has been a subject of intense research throughout the 3rd Millennium. Now that a general picture about microbiota composition in health and disease is emerging, questions about factors determining development of microbiotas with specific community structures will be addressed. To this end, usage of murine models for colonization studies remains crucial. Optical in vivo imaging of either bioluminescent or fluorescent bacteria is the basis for non-invasive detection of intestinal colonization of bacteria. Although recent advances in in vivo fluorescence imaging have overcome many limitations encountered in bioluminescent imaging of intestinal bacteria, such as requirement for live cells, high signal attenuation and 2D imaging, the method is still restricted to bacteria for which molecular cloning tools are available., Results: Here, we present usage of a lipophilic fluorescent dye together with Katushka far-red fluorescent protein to establish a dual-color in vivo imaging system to monitor GI transit of different bacterial strains, suitable also for strains resistant to genetic labeling. Using this system, we were able to distinguish two different E. coli strains simultaneously and show their unique transit patterns. Combined with fluorescence molecular tomography, these distinct strains could be spatially and temporally resolved and quantified in 3D., Conclusions: Developed novel method for labeling microbes and identify their passage both temporally and spatially in vivo makes now possible to monitor all culturable bacterial strains, also those that are resistant to conventional genetic labeling.

Published

2019