TY - JOUR A1 - Tian, Yuehui A1 - Yang, Shang A1 - Gao, Shiqiang T1 - Advances, perspectives and potential engineering strategies of light-gated phosphodiesterases for optogenetic applications JF - International Journal of Molecular Sciences N2 - The second messengers, cyclic adenosine 3′-5′-monophosphate (cAMP) and cyclic guanosine 3′-5′-monophosphate (cGMP), play important roles in many animal cells by regulating intracellular signaling pathways and modulating cell physiology. Environmental cues like temperature, light, and chemical compounds can stimulate cell surface receptors and trigger the generation of second messengers and the following regulations. The spread of cAMP and cGMP is further shaped by cyclic nucleotide phosphodiesterases (PDEs) for orchestration of intracellular microdomain signaling. However, localized intracellular cAMP and cGMP signaling requires further investigation. Optogenetic manipulation of cAMP and cGMP offers new opportunities for spatio-temporally precise study of their signaling mechanism. Light-gated nucleotide cyclases are well developed and applied for cAMP/cGMP manipulation. Recently discovered rhodopsin phosphodiesterase genes from protists established a new and direct biological connection between light and PDEs. Light-regulated PDEs are under development, and of demand to complete the toolkit for cAMP/cGMP manipulation. In this review, we summarize the state of the art, pros and cons of artificial and natural light-regulated PDEs, and discuss potential new strategies of developing light-gated PDEs for optogenetic manipulation. KW - cyclic nucleotides KW - phosphodiesterases (PDEs) KW - optogenetics KW - cAMP KW - cGMP Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-236203 SN - 1422-0067 VL - 21 IS - 20 ER - TY - JOUR A1 - Jessen, Christina A1 - Kreß, Julia K. C. A1 - Baluapuri, Apoorva A1 - Hufnagel, Anita A1 - Schmitz, Werner A1 - Kneitz, Susanne A1 - Roth, Sabine A1 - Marquardt, André A1 - Appenzeller, Silke A1 - Ade, Casten P. A1 - Glutsch, Valerie A1 - Wobser, Marion A1 - Friedmann-Angeli, José Pedro A1 - Mosteo, Laura A1 - Goding, Colin R. A1 - Schilling, Bastian A1 - Geissinger, Eva A1 - Wolf, Elmar A1 - Meierjohann, Svenja T1 - The transcription factor NRF2 enhances melanoma malignancy by blocking differentiation and inducing COX2 expression JF - Oncogene N2 - The transcription factor NRF2 is the major mediator of oxidative stress responses and is closely connected to therapy resistance in tumors harboring activating mutations in the NRF2 pathway. In melanoma, such mutations are rare, and it is unclear to what extent melanomas rely on NRF2. Here we show that NRF2 suppresses the activity of the melanocyte lineage marker MITF in melanoma, thereby reducing the expression of pigmentation markers. Intriguingly, we furthermore identified NRF2 as key regulator of immune-modulating genes, linking oxidative stress with the induction of cyclooxygenase 2 (COX2) in an ATF4-dependent manner. COX2 is critical for the secretion of prostaglandin E2 and was strongly induced by H\(_2\)O\(_2\) or TNFα only in presence of NRF2. Induction of MITF and depletion of COX2 and PGE2 were also observed in NRF2-deleted melanoma cells in vivo. Furthermore, genes corresponding to the innate immune response such as RSAD2 and IFIH1 were strongly elevated in absence of NRF2 and coincided with immune evasion parameters in human melanoma datasets. Even in vitro, NRF2 activation or prostaglandin E2 supplementation blunted the induction of the innate immune response in melanoma cells. Transcriptome analyses from lung adenocarcinomas indicate that the observed link between NRF2 and the innate immune response is not restricted to melanoma. KW - NRF2 KW - melanoma malignancy KW - COX2 expression Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-235064 SN - 0950-9232 VL - 39 ER - TY - THES A1 - Pickel, Simone T1 - Role of the β subunit of L-type calcium channels in cardiac hypertrophy T1 - Die Rolle der β Untereinheit von L-Typ Kalziumkänalen in der kardialen Hypertrophie N2 - L-type calcium channels (LTCCs) control crucial physiological processes in cardiomyocytes such as the duration and amplitude of action potentials, excitation-contraction coupling and gene expression, by regulating the entry of Ca2+ into the cells. Cardiac LTCCs consist of one pore-forming α1 subunit and the accessory subunits Cavβ, Cavα2δ and Cavγ. Of these auxiliary subunits, Cavβ is the most important regulator of the channel activity; however, it can also have LTCC-independent cellular regulatory functions. Therefore, changes in the expression of Cavβ can lead not only to a dysregulation of LTCC activity, but also to changes in other cellular functions. Cardiac hypertrophy is one of the most relevant risk factors for congestive heart failure and depends on the activation of calcium-dependent prohypertrophic signaling pathways. However, the role of LTCCs and especially Cavβ in this pathology is controversial and needs to be further elucidated. Of the four Cavβ isoforms, Cavβ2 is the predominant one in cardiomyocytes. Moreover, there are five different splice variants of Cavβ2 (Cavβ2a-e), differing only in the N-terminal region. We reported that Cavβ2b is the predominant variant expressed in the heart. We also revealed that a pool of Cavβ2 is targeted to the nucleus in cardiomyocytes. The expression of the nuclear Cavβ2 decreases during in vitro and in vivo induction of cardiomyocyte hypertrophy and overexpression of a nucleus-targeted Cavβ2 completely abolishes the in vitro induced hypertrophy. Additionally, we demonstrated by shRNA-mediated protein knockdown that downregulation of Cavβ2 enhances the hypertrophy induced by the α1-adrenergic agonist phenylephrine (PE) without involvement of LTCC activity. These results suggest that Cavβ2 can regulate cardiac hypertrophy through LTCC-independent pathways. To further validate the role of the nuclear Cavβ2, we performed quantitative proteome analyses of Cavβ2-deficient neonatal rat cardiomyocytes (NRCs). The results show that downregulation of Cavβ2 influences the expression of various proteins, including a decrease of calpastatin, an inhibitor of the calcium-dependent cysteine protease calpain. Moreover, downregulation of Cavβ2 during cardiomyocyte hypertrophy drastically increases calpain activity as compared to controls after treatment with PE. Finally, the inhibition of calpain by calpeptin abolishes the increase in PE-induced hypertrophy in Cavβ2-deficient cells. These results suggest that nuclear Cavβ2 has Ca2+- and LTCC-independent functions during the development of hypertrophy. Overall, our results indicate a new role for Cavβ2 in antihypertrophic signaling in cardiac hypertrophy. N2 - Durch die Regulation des Calciumeintritts in die Zellen kontrollieren L-Typ-Calciumkanäle (LTCCs) wichtige physiologische Prozesse wie die Dauer und Amplitude von Aktionspotentialen, die elektromechanische Kopplung und die Genexpression in Kardiomyozyten. Kardiale LTCCs bestehen aus einer porenformenden α1 Untereinheit und Hilfsuntereinheiten wie Cavβ, Cavα2δ und Cavγ. Von diesen Hilfsuntereinheiten ist Cavβ der wichtigste Regulator der Kanalfunktion, wobei Cavβ auch LTCC-unabhängige zelluläre und regulatorische Funktionen haben kann. Veränderungen in der Expression dieses Proteins können daher zu einer Fehlregulation der LTCC-Aktivität führen, jedoch auch zu Veränderungen von anderen zellulären Funktionen. Einer der häufigsten Risikofaktoren für kongestive Herzinsuffizienz ist die kardiale Hypertrophie, welche abhängig ist von der Aktivierung von Calcium-abhängigen prohypertrophen Signalwegen. Die Rolle von LTCCs und insbesondere von Cavβ in dieser Erkrankung ist jedoch kontrovers und muss noch weiter erforscht werden. Von den vier Cavβ Splicevarianten ist Cavβ2 die dominierende Form in Kardiomyozyten. Darüber hinaus existieren fünf verschiedene Splicevarianten von Cavβ2 (Cavβ2a-e), die sich jeweils nur in der N-terminalen Region unterscheiden. Wir konnten demonstrieren, dass von diesen Splicevarianten überwiegend Cavβ2b im Herzen exprimiert wird. Außerdem konnten wir zeigen, dass ein Teil von Cavβ2 im Nukleus von Kardiomyozyten zu finden ist. Die Expression von nuklearem Cavβ2 verringert sich während der in vitro und in vivo induzierten kardialen Hypertrophie und außerdem verhindert die Überexpression von im Kern lokalisiertem Cavβ2 die in vitro induzierte Hypertrophie komplett. Zusätzlich konnten wir demonstrieren, dass die Reduktion von Cavβ2 mittels shRNA zu einer Steigerung der Hypertrophie induziert durch die Stimulation mit dem α1-adrenergen Agonisten Phenylephrin (PE) führt, ohne dass die LTCC-Aktivität beteiligt ist. Diese Ergebnisse legen nahe, dass Cavβ2 die Entstehung von Hypertrophie durch LTCC-unabhängige Signalwege beeinflussen kann. Um die Rolle von nuklearem Cavβ2 zu bekräftigen, haben wir quantitative Proteomanalysen von Cavβ2 defizienten neonatalen Rattenkardiomyozyten (NRCs) durchgeführt. Die Ergebnisse zeigen, dass die Reduktion von Cavβ2 die Expression verschiedener Proteine beeinflusst, zum Beispiel wird Calpastatin, ein Inhibitor der calciumabhängigen Cysteinproteasen Calpain, herunterreguliert. Außerdem wird durch die Cavβ2 Reduktion während der Hypertrophie von Kardiomyozyten die Calpainaktivität verglichen mit den Kontrollen signifikant erhöht. Letztendlich konnten wir zeigen, dass die Inhibierung von Calpain durch Calpeptin die gesteigerte PE-induzierte Hypertrophie in Cavβ2-defizienten Zellen verhindert. Diese Ergebnisse lassen eine Calcium- und LTCC-unabhängige Funktion von nuklearem Cavβ2 während der Entwicklung von Hypertrophie, annehmen. Insgesamt deuten unsere Ergebnisse auf eine neue Rolle von Cavβ2 in den antihypertrophen Signalwegen in der kardialen Hypertrophie hin. KW - Herzhypertrophie KW - Calciumkanal KW - Herzmuskelzelle KW - L-type calcium channels KW - Cavβ subunit KW - Calpain KW - LTCC-independent function of Cavβ Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-192829 ER - TY - JOUR A1 - Capetian, Philipp A1 - Müller, Lorenz A1 - Volkmann, Jens A1 - Heckmann, Manfred A1 - Ergün, Süleyman A1 - Wagner, Nicole T1 - Visualizing the synaptic and cellular ultrastructure in neurons differentiated from human induced neural stem cells - an optimized protocol JF - International Journal of Molecular Sciences N2 - The size of the synaptic subcomponents falls below the limits of visible light microscopy. Despite new developments in advanced microscopy techniques, the resolution of transmission electron microscopy (TEM) remains unsurpassed. The requirements of tissue preservation are very high, and human post mortem material often does not offer adequate quality. However, new reprogramming techniques that generate human neurons in vitro provide samples that can easily fulfill these requirements. The objective of this study was to identify the culture technique with the best ultrastructural preservation in combination with the best embedding and contrasting technique for visualizing neuronal elements. Two induced neural stem cell lines derived from healthy control subjects underwent differentiation either adherent on glass coverslips, embedded in a droplet of highly concentrated Matrigel, or as a compact neurosphere. Afterward, they were fixed using a combination of glutaraldehyde (GA) and paraformaldehyde (PFA) followed by three approaches (standard stain, Ruthenium red stain, high contrast en-bloc stain) using different combinations of membrane enhancing and contrasting steps before ultrathin sectioning and imaging by TEM. The compact free-floating neurospheres exhibited the best ultrastructural preservation. High-contrast en-bloc stain offered particularly sharp staining of membrane structures and the highest quality visualization of neuronal structures. In conclusion, compact neurospheres growing under free-floating conditions in combination with a high contrast en-bloc staining protocol, offer the optimal preservation and contrast with a particular focus on visualizing membrane structures as required for analyzing synaptic structures. KW - transmission electron microscopy KW - human neurons KW - induced neural stem cells KW - synapse KW - synaptic vesicles KW - high contrast Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-236053 SN - 1422-0067 VL - 21 IS - 5 ER -