TY - JOUR A1 - Mantel, Frederick A1 - Müller, Elena A1 - Kleine, Philip A1 - Zimmermann, Marcus A1 - Exner, Florian A1 - Richter, Anne A1 - Weick, Stefan A1 - Ströhle, Serge A1 - Polat, Bülent A1 - Höcht, Stefan A1 - Flentje, Michael T1 - Chemoradiotherapy by intensity-modulated radiation therapy with simultaneous integrated boost in locally advanced or oligometastatic non-small-cell lung cancer-a two center experience JF - Strahlentherapie und Onkologie N2 - Purpose Integrating moderate hypofractionation to the macroscopic tumor with elective nodal irradiation while sparing the organs at risk (OAR) in chemoradiotherapy of locally advanced non-small-cell lung cancer. Methods From 2010-2018, treatment, patient and tumor characteristics of 138 patients from two radiation therapy centers were assessed. Chemoradiotherapy by intensity-modulated radiation therapy (IMRT) with a simultaneous integrated boost (SIB) to the primary tumor and macroscopic lymph node metastases was used. Results A total of 124 (90%) patients received concurrent chemotherapy. 106 (76%) patients had UICC (Union for International Cancer Control) stage ≥IIIB and 21 (15%) patients had an oligometastatic disease (UICC stage IV). Median SIB and elective total dose was 61.6 and 50.4 Gy in 28 fractions, respectively. Furthermore, 64 patients (46%) had an additional sequential boost to the primary tumor after the SIB-IMRT main series: median 6.6 Gy in median 3 fractions. The median cumulative mean lung dose was 15.6 Gy (range 6.2-29.5 Gy). Median follow-up and radiological follow-up for all patients was 18.0 months (range 0.6-86.9) and 16.0 months (range 0.2-86.9), respectively. Actuarial local control rates at 1, 2 and 3 years were 80.4, 68.4 and 57.8%. Median overall survival and progression-free survival was 30.0 months (95% confidence interval [CI] 23.5-36.4) and 12.1 months (95% CI 8.2-16.0), respectively. Treatment-related toxicity was moderate. Radiation-induced pneumonitis grade 2 and grade 3 occurred in 13 (9.8%) and 3 (2.3%) patients. Conclusions Chemoradiotherapy using SIB-IMRT showed promising local tumor control rates and acceptable toxicity in patients with locally advanced and in part oligometastatic lung cancer. The SIB concept, resulting in a relatively low mean lung dose, was associated with low numbers of clinically relevant pneumonitis. The overall survival appears promising in the presence of a majority of patients with UICC stage ≥IIIB disease. KW - local control KW - image-guided radiation therapy KW - thoracic cancer KW - hypofractionation KW - multimodal therapy Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-264821 SN - 1439-099X VL - 197 IS - 5 ER - TY - THES A1 - Ströhle, Serge - Peer T1 - Kultivierung von humanem Speicheldrüsengewebe in einer dreidimensionalen Polyurethanmatrix T1 - Cultivation of human salivary gland tissue in a three-dimensional Polyurethane Matrix N2 - Bei Tumoren von Kopf und Hals kann primär oder adjuvant durch Bestrahlung therapiert werden. Die Folgen dieser Behandlung können Xerostomie, Karies, Infektionen, Dysphagie oder Mundgeruch sein. Diese Nebenwirkungen vermindern die Lebensqualität des Patienten. Unterschiedliche Behandlungsansätze haben aufgrund von therapiebedingten Einschränkungen nicht den Weg in den klinischen Alltag gefunden. Eine Alternative zu den vorhandenen Behandlungsansätzen kann das Tissue Engineering sein. Das Ziel einer Normalisierung der Speichelproduktion nach Behandlung soll durch eine implantierbare, künstliche Speicheldrüse erreicht werden. Kann humanes natives Speicheldrüsengewebe der Parotis auf gradientenfreiem dreidimensional aufgebauten Polyurethan wachsen und seine Funktionalität beibehalten? Humane Parotiszellen wurden von 20 Patienten im Alter von 42 - 90 Jahren durch Operation entnommenen und in Polystyrol-Zellkulturflaschen mit dem Nährmedium BEGM herangezüchtet. Es erfolgte eine 2D-Zellverteilung der reinen Parotiskultur. Zur Kontrolle der Vitalität zwischen den Passagen wurde eine Trypan-Blau Färbung verwendet. Als Trägermaterial der Zellen wurde eine biokompatible, abbaubare Matrix aus ε-Polycaprolacton verarbeitet. Die Übertragung der humanen Parotiszellen wurde mit einer Kleberproteinlösung, bestehend aus den Hauptbestandteilen Aprotinin, Fibrinogen und der Thrombinlösung durchgeführt. 7,14 und 21 Tage nach Aufbringung wurde der Überstand der zeitgleich entnommenen Konstrukte zur Überprüfung des α-Amylase konserviert. Zusätzlich wurden an den 3 Untersuchungstagen Konstrukte für die Anfertigung von histologischen Schnitten, quantitativer PCR, indirekter Immunfluoreszenz und zur Elektronenmikroskopie entnommen. Zur Überprüfung der Funktionalität der angezüchteten Speicheldrüsenzellen wurde das Enzym α-Amylase und das Wasserkanalprotein Aquaporin 5 herangezogen. Bei der Kultivierung der humanen Speicheldrüsenzellen konnte durch den Vitalitätstest Trypan-Blau Färbung in Kombination mit einer Neubauerzählkammer eine konstant hohe Anzahl an vitalen Zellen bis zur 4. Passage nachgewiesen werden. Durch die Lebend/Tot Färbung auf FDA/EB Basis der Konstrukte über die Untersuchungszeit von 14 Tagen konnte keine Vermehrung von avitalen Zellen mikroskopisch festgestellt werden. Die statistische Auswertung mittels Boxplots des ELISA berechnete für den ersten Untersuchungstag einen Median auf niedrigem Niveau von 4,4 U/l und sank im weiteren Zeitverlauf am Untersuchungstag 21 auf die niedrigsten Median von 2,2 U/l ab. α-Amylase konnte an allen 3 Tagen mittels quantitativer PCR und indirekter Immunfluoreszenz belegt werden. Aquaporin 5 als Funktionsnachweis war in der vorliegenden Studie nicht signifikant durch quantitative PCR beweisbar. Die Rasterelektronenmikroskopie bildete adhärente Zellen in kugeliger Form aus den besiedelten Matrices nach 7 Tagen Kultivierung ab. Durch die Transmissionselektronenmikroskopie konnten Zellen, die Zellfortsätze ausgebildet hatten nach 14 Tagen beobachtet werden. Der Versuch, histologische Schnitte auf Grundlage der Paraffineinbettung oder Kryo-Konservierung zu erzeugen, musste frustran abgeschlossen werden. Eine Kultivierung von Speicheldrüsenzellen auf einer Matrix aus ε-Polycaprolacton ohne Gradienten ist eingeschränkt umsetzbar. Die Studie konnte zeigen, dass das Wachstum der Zellen auf konstant niedrigem Niveau über den Untersuchungszeitraum von 21 Tagen lag. Der Funktionsnachweis von α-Amylase auf absinkendem niedrigem Niveau sowie fehlender Bestätigung von Aquaporin 5 kann als stationäre Phase des Wachstums interpretiert werden. Zur Verbesserung der Zellentwicklung sollte die besiedelte Matrix zu einem 3D-Zellwachstum anregen. Bei sequenziell entstehender Polarität der Zellen käme es zu einer Verbesserung der Vitalität sowie der vermehrten Ausbildung von α-Amylase und Aquaporin 5. Dies könnte in einer Kombination der Zellkultur aus Parotiszellen mit Kokulturen aus humanen Myoepithelzellen und Parenchymzellen erreicht werden. Sehr gute Ergebnisse des Zellwachstums und der Zellfunktion konnten aktuell in anderen Studien auf der Trägersubstanz Matrigel oder durch Rebesiedelung von dezellularisierten Organen beobachtet werden. N2 - In the case of tumours of the head and neck, the tumour can be treated primarily or adjuvantly by radiation. The consequences of this treatment can be xerostomia, caries, infections, dysphagia or bad breath. These side effects reduce the patient's quality of life. Different treatment approaches have not found their way into the clinical routine due to therapy related limitations. Tissue engineering can be an alternative to the existing treatment approaches. The goal of normalising saliva production after treatment is to be achieved by means of an implantable, artificial salivary gland. Can human native salivary gland tissue of the parotid gland grow on gradient-free three-dimensional polyurethane and retain its functionality? Human parotid gland cells were taken from 20 patients aged 42 - 90 years by surgery and cultivated in polystyrene cell culture bottles with the culture medium BEGM. A 2D cell distribution of the pure parotid culture was performed. A trypan-blue staining was used to control the vitality between the passages. A biocompatible, degradable matrix of ε-polycaprolactone was used as carrier material for the cells. The transfer of human parotid cells was performed with a glue protein solution consisting of the main components aprotinin, fibrinogen and the thrombin solution. 7, 14 and 21 days after application, the supernatant of the constructs taken at the same time was preserved for the examination of α amylase. In addition, constructs for the preparation of histological sections, quantitative PCR, indirect immunofluorescence and electron microscopy were taken during the 3 days of examination. The enzyme α-amylase and the water channel protein aquaporin 5 were added to test the functionality of the cultivated salivary gland cells. During the cultivation of human salivary gland cells, the vitality test Trypan blue staining in combination with a Neubauer counting chamber showed a constantly high number of vital cells up to the 4th passage. The live/dead staining on FDA/EB basis of the constructs over the examination period of 14 days did not show any proliferation of avital cells. The statistical evaluation by means of ELISA box plots calculated a median at a low level of 4.4 U/l for the first day of the examination and dropped to the lowest median of 2.2 U/l on examination day 21. α-amylase was detected on all 3 days by quantitative PCR and indirect immunofluorescence. Aquaporin 5 as a functional test was not significantly detectable by quantitative PCR in this study. The scanning electron microscopy imaged adherent cells in spherical form from the colonised matrices after 7 days of cultivation. Using transmission electron microscopy, cells that had formed cell extensions could be observed after 14 days. The attempt to produce histological sections based on paraffin embedding or cryopreservation had to be frustrated. Cultivation of salivary gland cells on a matrix of ε-polycaprolactone without gradients is of limited use. The study was able to show that the growth of the cells was at a constantly low level over the 21-day period of the study. The proof of function of α-amylase at a decreasing low level and the lack of confirmation of aquaporin 5 can be interpreted as a stationary phase of growth. To improve cell development, the colonised matrix should stimulate 3D cell growth. If the cells were to develop a sequential polarity, there would be an improvement in vitality as well as increased formation of α-amylase and aquaporin 5. This could be achieved by a combination of cell culture from parotid cells with cocultures of human myoepithelial cells and parenchymal cells. Very good results of cell growth and cell function could be observed in other studies on the carrier substance Matrigel or by re-colonisation of decellularised organs. KW - Ohrspeicheldrüse KW - Tissue Engineering KW - Polyurethane KW - Trägersubstanz KW - Zellkultur KW - Ohrspeicheldrüse KW - Elektronenmikroskopie KW - Biomarker KW - Real time quantitative PCR KW - Electron microscopy KW - Cell culture KW - Parotid glands KW - Biochemical markers KW - Quantitative Real-Time PCR Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-216887 ER - TY - JOUR A1 - Weick, Stefan A1 - Breuer, Kathrin A1 - Richter, Anne A1 - Exner, Florian A1 - Ströhle, Serge-Peer A1 - Lutyj, Paul A1 - Tamihardja, Jörg A1 - Veldhoen, Simon A1 - Flentje, Michael A1 - Polat, Bülent T1 - Non-rigid image registration of 4D-MRI data for improved delineation of moving tumors JF - BMC Medical Imaging N2 - Background To increase the image quality of end-expiratory and end-inspiratory phases of retrospective respiratory self-gated 4D MRI data sets using non-rigid image registration for improved target delineation of moving tumors. Methods End-expiratory and end-inspiratory phases of volunteer and patient 4D MRI data sets are used as targets for non-rigid image registration of all other phases using two different registration schemes: In the first, all phases are registered directly (dir-Reg) while next neighbors are successively registered until the target is reached in the second (nn-Reg). Resulting data sets are quantitatively compared using diaphragm and tumor sharpness and the coefficient of variation of regions of interest in the lung, liver, and heart. Qualitative assessment of the patient data regarding noise level, tumor delineation, and overall image quality was performed by blinded reading based on a 4 point Likert scale. Results The median coefficient of variation was lower for both registration schemes compared to the target. Median dir-Reg coefficient of variation of all ROIs was 5.6% lower for expiration and 7.0% lower for inspiration compared with nn-Reg. Statistical significant differences between the two schemes were found in all comparisons. Median sharpness in inspiration is lower compared to expiration sharpness in all cases. Registered data sets were rated better compared to the targets in all categories. Over all categories, mean expiration scores were 2.92 +/- 0.18 for the target, 3.19 +/- 0.22 for nn-Reg and 3.56 +/- 0.14 for dir-Reg and mean inspiration scores 2.25 +/- 0.12 for the target, 2.72 +/- 215 0.04 for nn-Reg and 3.78 +/- 0.04 for dir-Reg. Conclusions In this work, end-expiratory and inspiratory phases of a 4D MRI data sets are used as targets for non-rigid image registration of all other phases. It is qualitatively and quantitatively shown that image quality of the targets can be significantly enhanced leading to improved target delineation of moving tumors. KW - 4D-MRI KW - Non-rigid image registration KW - Radiotherapy treatment planning KW - Respiratory induced tumor motion Y1 - 2020 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:bvb:20-opus-229271 VL - 20 ER -