@article{KreftHughes1982, author = {Kreft, J{\"u}rgen and Hughes, Colin}, title = {Cloning vectors derived from plasmids and phage of Bacillus}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-47014}, year = {1982}, abstract = {No abstract available}, language = {en} } @article{DandekarTollervey1989, author = {Dandekar, Thomas and Tollervey, David}, title = {Cloning of Schizosaccharomyces pombe genes encoding the U1,U2,U3 and U4 snRNAs}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-29919}, year = {1989}, abstract = {No abstract available}, language = {en} } @techreport{GesslerSimolaBruns1989, author = {Gessler, Manfred and Simola, Kalle O. and Bruns, Gail A. P.}, title = {Cloning of breakpoints of a chromosome translocation identifies the AN2 locus}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-30177}, year = {1989}, abstract = {Chromosome translocations involving llpl3 have been associated with familial aniridia in two kindreds highlighting the chromosomal localization of the AN2 locus. This locus is also part of the WAGR complex (Wilros tumor, aniridia, genitourinary abnormalities, and mental retardation). In one kindred, the translocation is associated with a deletion, and probes for this region were used to identify and clone the breakpoints of the translocation in the second kindred. Comparison of phage restriction maps exclude the presence of any sizable deletion in this case. Sequences at the chromosome 11 breakpoint are conserved in multiple species, suggesting that the translocation falls within the AN2 gene.}, language = {en} } @phdthesis{Stojic2005, author = {Stojic, Jelena}, title = {Cloning and functional characterization of novel genes expressed preferentially in the human retina}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-13746}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2005}, abstract = {The human retina is a multi-layered neuronal tissue specialized for the reception and processing of visual information. The retina is composed of a great diversity of neuronal cell types including rod and cone photoreceptors, bipolar cells, ganglion cells, amacrine cells, horizontal cells and M{\"u}ller glia. In response to light, a coordinated series of molecular events, the so-called phototransduction cascade, is triggered in photoreceptor cells and the signals from the photoreceptors are further processed by the bipolar and ganglion cells to the higher centers of the brain. The retina as highly complex system may be greatly susceptible to genetic defects which can lead to a wide range of disease phenotypes. Therefore, isolation and characterisation of the genes active in the human retina will facilitate our deeper understanding of retinal physiology and mechanisms underlying retinal degeneration and provide novel candidates for the retinal disease genes. To identify novel genes that are specifically or predominantly expressed in the human retina, a cDNA library enriched for retina specific transcripts was generated using suppression subtractive hybridization (SSH) technique. In total, 1113 clones were randomly isolated from the retina SSH cDNA library and partially sequenced. On the basis of BLASTN algorithm analysis these clones were classified into four categories including those with I) significant homology to known human genes (766/1113), II) significant homology to partial transcripts and hypothetical gene predictions (162/1113), III) no homology to known mRNAs (149/1113), and IV) vector sequences and clones derived from mitochondrial genes (36/1113). After correcting for redundancy, category I represented 234 known human genes and category II a total of 92unknown transcripts. Clones from category I, were selected for expression analysis by RT-PCR in a great number of human tissues. This resulted in the identification of 16 genes which were expressed exclusively in the retina, 13 which were highly expressed in the retina compared to other tissues, 12 genes which were specifically expressed in neuronal tissues and 48 ubiquitously expressed genes. Thus, our expression analysis resulted in the identification of 29 genes exclusively or abundantly transcribed in the human retina. Of those, retina specific genes L25,L33, L35, L37, L38 and L40 were selected for further analysis. To characterize the complete mRNA sequences of these transcripts a full-length human retina cDNA library was constructed. The analysis of the L25 gene revealed three splicing variants of the ABCC5 gene, consequently named ABCC5_SV1 (SV1), ABCC5_SV2 (SV2) and ABCC5_SV3 (SV3).These isoforms comprise the first five exons of ABCC5 and additional novel exons named 5a, 5b and 5c, generated by differential exon usage. The determined lengths of the three transcripts are 2039 bp, 1962 bp, and 1887 bp in size, respectively. RT-PCR, real-time PCR and Northern blot analysis of ABCC5 as well as the isoforms SV1, SV2 and SV3demonstrated high levels of expression for all transcripts in the retina compared to other tissues. Analysis of their nucleotide sequences revealed that inclusion of exon 5a in splicing variant SV1 produced a frame shift and premature termination codon (PTC). Our data show that this splice variant is the target of nonsense mediated mRNA decay (NMD). This was shown by inhibition of protein synthesis with antibiotics puromycin and anisomycin in human cell lines A-RPE 19 and Y79. Our analysis resulted in an increase of the PTC containing transcript and a decrease of the ABCC5 transcript. Conversely, the amount of both transcripts (SV1 and ABCC5) returned to pre-treatment levels after removal of the inhibitors. Together, our results suggest that alternative splicing of the ubiquitously expressed ABCC5 gene in addition to NMD is involved in retina-specific transcriptional regulation of the mRNA level of ABCC5. In contrast, additional experiments demonstrated that the levels of expression ofSV2 and SV3 isoforms do not appear to influence ABCC5 transcription. Several of the cloned genes were selected for additional genotyping of single nucleotide polymorphisms (SNPs) in order to construct their SNP maps which are going to be used for future association studies of complex disease AMD. Thus, identification of novel retinal genes and their functional characterization will further our elucidation of retinal physiology in general and in the diseased state in particular, by providing candidate retinal disease genes.}, subject = {Netzhaut}, language = {en} } @article{GabelliniHarnischMcCarthyetal.1985, author = {Gabellini, N. and Harnisch, U. and McCarthy, J. E. and Hauska, G. and Sebald, Walter}, title = {Cloning and expression of the fbc operon encoding the FeS protein, cytochrome b and cytochrome c\(_1\) from the Rhodopseudomonas sphaeroides b/c\(_1\) complex}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-62642}, year = {1985}, abstract = {The gene for the FeS protein of the Rhodopseudomonas sphaeroides b/c1 complex was identified by means of crosshybridization with a segment of the gene encoding the corresponding FeS protein of Neurospora crassa. Plasmids (pRSF1-14) containing the cross-hybridizing region, covering in total 13.5 kb of chromosomal DNA, were expressed in vitro in a homologous system. One RSF plasmid directed the synthesis of all three main polypeptides of the R. sphaeroides blc1 complex: the FeS protein, cytochrome b and cytochrome c1• The FeS protein and cytochrome c1 were apparently synthesized as precursor fonns. None of the pRSF plasmids directed the synthesis of the 10-kd polypeptide found in b/c1 complex preparations. Partial sequencing of the cloned region was performed. Several sites of strong homology between R. sphaeroides and eukaryotic polypeptides of the b/c1 complex were identified. The genes encode the three b/c1 polypeptides in the order: (5') FeS protein, cytochrome b, cytochrome c1• The three genes are transcribed to give a polycistronic mRNA of 2.9 kb. This transcriptional unit has been designated the jbc operon; its coding capacity corresponds to the size of the polycistronic mRNA assuming that only the genes for the FeS protein (jbcF), cytochrome b (jbcß) and cytochrome c1 (jbcC) are present. This could indicate that these three subunits constitute the minimal catalytic unit of the b/c1 complex from photosynthetic membranes.}, subject = {Biochemie}, language = {en} } @article{KreftBergerHaertleinetal.1983, author = {Kreft, J{\"u}rgen and Berger, Harald and H{\"a}rtlein, Michael and M{\"u}ller, Bodo and Weidinger, Gerhard and Goebel, Werner}, title = {Cloning and expression in Escherichia coli and Bacillus subtilis of the hemolysin (cereolysin) determinant from Bacillus cereus}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-60596}, year = {1983}, abstract = {From a cosmid gene bank of Bacillus cereus GP4 in Escherichia coli we isolated clones which, after several days of incubation, formed hemolysis zones on erythrocyte agar plates. These clones contained recombinant cosmids with B. cereus DNA insertions of varying lengths which shared some common restriction fragments. The smallest insertionwas recloned as aPstl fragment into pJKK3-1, a shuttle vector which rep{\"u}cates in Bacillus subtilis and E. coli. When this recombinant plasmid (pJKK3-1 hly-1) was transformed into E. coli, it caused hemolysis on erythrocyte agar plates, but in liquid assays no extemal or intemal hemolytic activity could be detected with the E. coli transformants. B. subtilis carrying the same plasmid exhibited hemolytic activity at Ievels comparable to those ofthe B. cereus donor strain. The hemolysin produced in B. subtilis seemed to be indistinguishable from cereolysin in its sensitivity to cholesterol, activation by dithiothreitol, and inactivation by antibodies raised against cereolysin. When the recombinant DNA carrying the cereolysin gene was used as a probe in hybridization experiments with chromosomal DNA from a streptolysin 0-producing strain of Streptococcus pyogenes or from {\"u}steriolysin-producing strains of Usteria monoeytogenes, no positive hybridization signals were obtained. These data soggest that the genes for these three SH-activated cytolysins do not have extended sequence homology.}, subject = {Biologie}, language = {en} } @phdthesis{Mao2006, author = {Mao, Zhengrong}, title = {Clonality analysis in B-Cell Chronic Lymphocytic Leukemia (B-CLL) associated with Richter's syndrome}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-20596}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2006}, abstract = {Die chronische lymphatische Leuk{\"a}mie vom B-Zell-Typ (B-CLL) macht ca. 90\% der chronischen lymphatischen Leuk{\"a}mien aus. Der klinische Verlauf der B-CLL ist heterogen, und bei 3-5\% der Patienten kommt es im Verlauf der Erkrankung zu einer Transformation in ein aggressives Lymphom, meist in ein diffuses großzelliges B-Zell-Lymphom (DLBCL) oder in ein Hodgkin-Lymphom (HL). Eine solche Transformation wird als Richter-Syndrom bezeichnet und ist mit einer ung{\"u}nstigen klinischen Prognose assoziiert. In B-Zell-Lymphomen (B-NHL) erm{\"o}glicht der Mutationsstatus der variablen Anteile der Immunglobulinschwerkettengene (IgVH) eine Aussage {\"u}ber das Entwicklungsstadium der B-Zelle, in dem sich die Transformation zu einem B-Zell-Lymphom ereignet hat. In der B-CLL stellt der Mutationsstatus auch einen bedeutenden prognostischen Faktor dar, wobei die Erkrankung bei Patienten mit unmutierten IgVH Genen meist einen ung{\"u}nstigen klinischen Verlauf zeigt. Die wenigen bisher durchgef{\"u}hrten molekularen Analysen an F{\"a}llen von Richter-Syndromen deuten darauf hin, dass ein Transformationsereignis sowohl bei B-CLL-Patienten mit mutierten als auch mit unmutierten IgVH Genen vorkommen kann, und dass die Tumorzellen des DLBCL oder HL sowohl klonal identisch mit dem B-CLL-Klon sein k{\"o}nnen als auch unabh{\"a}ngig als sekund{\"a}res Lymphom entstehen k{\"o}nnen. Um die klonale Beziehung zwischen DLBCL- bzw. Hodgkin/Reed-Sternberg (HRS)-Zellen und den Zellen der vorbestehenden B-CLL zu analysieren, den Mutationsstatus des IgVH Gens sowie m{\"o}gliche prognostische Faktoren in B-CLL-F{\"a}llen mit Richter-Transformation zu identifizieren, wurde eine gr{\"o}ßere Fallserie mit Hilfe eines PCR-basierten GeneScan Ansatzes mit anschließender Sequenzierung der IgVH-Gene untersucht. In F{\"a}llen mit HRS bzw. HRS-{\"a}hnlichen Zellen wurden die CD30-positiven Tumorzellen mittels Laser-Capture Mikrodissektion (LCM) isoliert. Weiterhin erfolgte eine morphologische und immunhistochemische Analyse der F{\"a}lle. Insgesamt wurden 48 Patientenproben untersucht, darunter 40 F{\"a}lle mit Richter-Syndrom sowie weitere 8 B-CLL-F{\"a}lle mit CD30-positiven HRS-{\"a}hnlichen Zellen. Unter den 40 Proben mit Richter-Syndrom zeigten 34 B-CLL-F{\"a}lle eine Transformation in ein DLBCL, in 6 F{\"a}llen erfolgte eine Transformation in ein HL. In 23 F{\"a}llen mit B-CLL und DLBCL wurde eine Sequenzierung der IgVH Gene durchgef{\"u}hrt. In 18 F{\"a}llen waren B-CLL und DLBCL klonal identisch, in 5 F{\"a}llen war das DLBCL als klonal unabh{\"a}ngige Neoplasie entstanden. Unter den klonal verwandten Paaren zeigten 11 von 15 Paaren unmutierte IgVH-Gene sowohl in der B-CLL als auch im DLBCL, wohingegen 5 von 6 F{\"a}lle mit Transformation einer B-CLL in ein HL mutierte IgVH Gene trugen. HRS-Zellen in 2 F{\"a}llen und HRS-{\"a}hnliche Zellen in einem Fall waren klonal verschieden vom B-CLL-Zellklon. Die VH-Gene VH3-23, VH3-74, VH1-2 und VH3-9 waren {\"u}berproportional h{\"a}ufig in B-CLL F{\"a}llen mit einer sp{\"a}teren Transformation in ein DLBCL vertreten, wohingegen VH4-34 und VH3-48 in mehr als der H{\"a}lfte der F{\"a}lle mit Transformation zu einem HL nachgewiesen werden konnten. Der immunhistochemische Nachweis von ZAP70 zeigte eine signifikante Assoziation mit unmutierten IgVH-Genen in B-CLL mit nachfolgender Richter-Transformation. Bei 24 Patienten konnte der klinische Verlauf eruiert werden. Die mediane {\"U}berlebenszeit von Patienten mit B-CLL mit stattgehabter Transformation in ein DLBCL oder ein HL betrug 7 beziehungsweise 21 Monate. Es fanden sich weder signifikante Unterschiede der {\"U}berlebenszeit zwischen klonal verwandten und nicht verwandten F{\"a}llen, noch zwischen IgVH-mutierten und -unmutierten F{\"a}llen. Zusammenfassend kann festgestellt werden, dass bei der Richter-Transformation einer B-CLL in ein DLBCL dieses einerseits aus dem pr{\"a}existenten B-CLL-Klon entstehen kann, andererseits aber auch als unabh{\"a}ngige, klonal nicht verwandte Neoplasie auftreten kann. In der Mehrzahl der F{\"a}lle (78\% in dieser Serie) sind B-CLL und DLBCL jedoch klonal identisch und nur gelegentlich entsteht ein DLBCL ohne klonale Beziehung zur B-CLL als unabh{\"a}ngige, sekund{\"a}re Neoplasie. Eine klonale Transformation in ein DLBCL tritt vorwiegend bei B-CLL-Patienten mit unmutierten IgVH-Genen auf, wohingegen die Mehrzahl der B-CLL-Patienten mit einer Transformation in ein HL oder CD30-positive HRS-{\"a}hnliche Zellen mutierte IgVH-Gene aufweist. Dieser Befund l{\"a}sst auf unterschiedliche Transformationswege der beiden Subtypen des Richter-Syndroms schließen. Weiterhin existieren vermutlich wesentliche Unterschiede in der Pathogenese zwischen DLBCL-F{\"a}llen, die sich aus einer vorbestehenden B-CLL entwickelt haben, und de novo DLBCL-F{\"a}llen, da de novo DLBCL zumeist durch mutierte IgVH-Gene charakterisiert sind.}, subject = {B-Zell-Leuk{\"a}mie}, language = {en} } @phdthesis{Goldau2002, author = {Goldau, Rainer}, title = {Clinical evaluation of novel methods to determine dialysis parameters using conductivity cells}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-3125}, school = {Universit{\"a}t W{\"u}rzburg}, year = {2002}, abstract = {During the last two decades an ongoing discussion about the necessary dose of dialysis brought the result that the urea based Kt/V value is significantly correlated to morbidity of the end stage renal disease (ESRD) patients. Even if it is not completely accepted, it seems to be more and more agreement of the nephrological community that for good dialysis practice Kt/V should be kept above 1.2 to 1.3 in the usual 3X4 hours per week dialysis schedule for patients without own residual clearance to assure long term quality of life, low morbidity and mortality. K is the clearance of urea the dialysis system can apply, t is the treatment time and V is the urea distribution volume of the patient, which is nearly equal to total body water. Kt/V has the unit of a drug dose (ml of drug per ml of patient volume) and therefore sometimes is called dialysis 'dose', even if this is subject of discussion because it implies that the dose can be described with only one urea related number. This work does not participate in this discussion. The premise of this work is more technical: Whatever the final result of the above discussion will be, a patient-friendly, precise cost-neutral and handy technical solution should be given to the hand of the interested nephrologist to continuously supervise the urea based Kt/V that is applied to the patient. Of course this is combined with the hope that the long term mortality can be decreased if a covering online dialysis success control is facilitated. The technical solution that has been chosen is based on the equivalence of the diffusion coefficients of sodium chloride and urea. It is central subject of the investigation if the diffusive behaviour of sodium is equal to that of urea crossing the dialysis filter membrane. The advantage that makes the principle so handy is that sodium can be measured very precise by standard conductivity cells as they are implemented in dialysis machines in large numbers. The only necessary hardware modification is a second conductivity cell downstream the dialyser to be able to measure the mass balance over the filter. This is more complicated with urea that can only be measured undergoing an enzymatic conversion to ammonium ions. The ammonium ions induce a membrane potential, which is measured with very sensitive amplifiers. A cooling chain for the enzyme must be maintained. To find and approve the conductivity based technical solution two in-vivo studies have been conducted. In the first study a conductivity step profile, varying the conductivity in static levels in a baseline - 7 min high - 7min low- baseline shape, was applied that can be utilised to measure the urea clearance very accurate. This principle has been described in 1982 in a patent application. In a sequence of 206 computer recorded dialysis sessions with 22 patients it was found that urea clearance could be electrolytically measured with a mean error+/-standard deviation of -1.46+/-4.75\% , n=494. The measurement of Kt/V according to a single pool model was of similar accuracy: 2.88+/-4.15\% . Although in accordance with other studies these findings at an average confirmed the high correlation of ionic and urea based clearance measurements, an effect was found that was not consistent with the theory that was existent so far. It was found in the first study that the accuracy of the step profile measurements were dependent of the size of the patient, in particular of the urea distribution volume. Moreover it was of relevance which part of the step profile was used: the high-low states, the baseline- low or the baseline-high states. This was a theoretical lack. Careful analysis led to the result that sodium transfer from and into the patient was the reason for the dependence. This led to the enhancement of the theory that seems to correctly describe the nature of the effect. A new demand now was to minimise the sodium transfer. This was limited using static step profiles because in the time it needs to become stable sodium is shifted. In consequence non-stable, dynamic short conductivity boli were developed that allowed to minimise the amount of sodium to be shifted to the limits of the technical resolution of the measurement systems. Also the associated mathematical tools to evaluate the boli had to be suited to the problem. After termination of this process a second study was conducted to approve the new method found. In this study with 10 patients and 93 sessions, 264 step profile measurements and 173 bolus ionic dialysance measurements it was found that the bolus measurements matched their related blood side urea clearance references with the outstanding accuracy of (error+/-SD) 0.06+/-4.76\%. The result was not significantly different (p=0.87) from the reference by student's t-test for paired data. The Kt/V reference according to the single pool variable volume urea kinetic model (sPVVUKM) was found to be matched by the bolus principle with 5.32+/-3.9\% accuracy and a correlation of 0.98. The remaining difference of 5.32\% can be attributed to the neglect of the urea generation rate. Also the step profile was found to be very precise here. The error versus sPVVUKM was 0.05\%+/-5\%, r=0.96. However it did not image the neglect of urea generation correctly. Also a two pool modelling that comprises an internal compartimentation of the fluid pools of the patient was applied to the continuously recorded data. This two pool urea kinetic model (2PUKM) is regarded to be a more precise theoretical approach and now includes the urea generation. It found the bolus principle to deviate -3.04 +/- 14.3\%, n.s., p=0.13. The high standard deviation is due to the complexity of the model. Further from the developed theory a simplified method to roughly measure the sodium distribution volume could be derived. This method was tested in-vitro versus a container with dialysate of known volume and in-vivo versus the urea distribution volume. The in-vitro results were -19.9+/-34\%, r=0.92, n.s, p=0.916. In-vivo they were found to be -7.4+/-23.2\%, r=0.71, n.s., p=0.39. Due to dilution theory the sodium and urea distribution volumes virtually appear to be very similar using this method, although they absolutely differ significantly. Facing the strong simplifications that were made before applying this theory these results seem to be very encouraging that it could be possible to develop a principle to measure not only K but also V electrolytically. This would allow a true Kt/V measurement. The empirical urea distribution volume measurement using anthropometrical formulas has been compared to analytical methods. It has been found that the use Watson's formula with a -13\% correction gives good results. The correction should be applied with great care because it increases Kt/V just on a arithmetical base to the disadvantage of the patient. Also electrolytical plasma sodium measurement was evaluated and can be measured using a mixed analytic-empirical formula with an accuracy of 4.3+/-1.2\%. In summary, conductivity based methods seem to be a convenient method to measure several dialysis parameters of some clinical interest without effort. The results of this work meanwhile are implemented with substantial numbers into commonly available dialysis machines and the experience of the first time shows that the principle is well accepted by the clinicians.}, subject = {H{\"a}modialyse}, language = {en} } @article{GebertSteffanDewenterMorettoetal.2019, author = {Gebert, Friederike and Steffan-Dewenter, Ingolf and Moretto, Philippe and Peters, Marcell K.}, title = {Climate rather than dung resources predict dung beetle abundance and diversity along elevational and land use gradients on Mt. Kilimanjaro}, series = {Journal of Biogeography}, volume = {47}, journal = {Journal of Biogeography}, number = {2}, doi = {10.1111/jbi.13710}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-204701}, pages = {371 -- 381}, year = {2019}, abstract = {Aim: While elevational gradients in species richness constitute some of the best depicted patterns in ecology, there is a large uncertainty concerning the role of food resource availability for the establishment of diversity gradients in insects. Here, we analysed the importance of climate, area, land use and food resources for determining diversity gradients of dung beetles along extensive elevation and land use gradients on Mt. Kilimanjaro, Tanzania. Location: Mt. Kilimanjaro, Tanzania. Taxon: Scarabaeidae (Coleoptera). Methods: Dung beetles were recorded with baited pitfall traps at 66 study plots along a 3.6 km elevational gradient. In order to quantify food resources for the dung beetle community in form of mammal defecation rates, we assessed mammalian diversity and biomass with camera traps. Using a multi-model inference framework and path analysis, we tested the direct and indirect links between climate, area, land use and mammal defecation rates on the species richness and abundance of dung beetles. Results: We found that the species richness of dung beetles declined exponentially with increasing elevation. Human land use diminished the species richness of functional groups exhibiting complex behaviour but did not have a significant influence on total species richness. Path analysis suggested that climate, in particular temperature and to a lesser degree precipitation, were the most important predictors of dung beetle species richness while mammal defecation rate was not supported as a predictor variable. Main conclusions: Along broad climatic gradients, dung beetle diversity is mainly limited by climatic factors rather than by food resources. Our study points to a predominant role of temperature-driven processes for the maintenance and origination of species diversity of ectothermic organisms, which will consequently be subject to ongoing climatic changes.}, language = {en} } @article{UphusLuepkeYuanetal.2021, author = {Uphus, Lars and L{\"u}pke, Marvin and Yuan, Ye and Benjamin, Caryl and Englmeier, Jana and Fricke, Ute and Ganuza, Cristina and Schwindl, Michael and Uhler, Johannes and Menzel, Annette}, title = {Climate effects on vertical forest phenology of Fagus sylvatica L., sensed by Sentinel-2, time lapse camera, and visual ground observations}, series = {Remote Sensing}, volume = {13}, journal = {Remote Sensing}, number = {19}, issn = {2072-4292}, doi = {10.3390/rs13193982}, url = {http://nbn-resolving.de/urn:nbn:de:bvb:20-opus-248419}, year = {2021}, abstract = {Contemporary climate change leads to earlier spring phenological events in Europe. In forests, in which overstory strongly regulates the microclimate beneath, it is not clear if further change equally shifts the timing of leaf unfolding for the over- and understory of main deciduous forest species, such as Fagus sylvatica L. (European beech). Furthermore, it is not known yet how this vertical phenological (mis)match — the phenological difference between overstory and understory — affects the remotely sensed satellite signal. To investigate this, we disentangled the start of season (SOS) of overstory F.sylvatica foliage from understory F. sylvatica foliage in forests, within nine quadrants of 5.8 × 5.8 km, stratified over a temperature gradient of 2.5 °C in Bavaria, southeast Germany, in the spring seasons of 2019 and 2020 using time lapse cameras and visual ground observations. We explained SOS dates and vertical phenological (mis)match by canopy temperature and compared these to Sentinel-2 derived SOS in response to canopy temperature. We found that overstory SOS advanced with higher mean April canopy temperature (visual ground observations: -2.86 days per °C; cameras: -2.57 days per °C). However, understory SOS was not significantly affected by canopy temperature. This led to an increase of vertical phenological mismatch with increased canopy temperature (visual ground observations: +3.90 days per °C; cameras: +2.52 days per °C). These results matched Sentinel-2-derived SOS responses, as pixels of higher canopy height advanced more by increased canopy temperature than pixels of lower canopy height. The results may indicate that, with further climate change, spring phenology of F. sylvatica overstory will advance more than F. sylvatica understory, leading to increased vertical phenological mismatch in temperate deciduous forests. This may have major ecological effects, but also methodological consequences for the field of remote sensing, as what the signal senses highly depends on the pixel mean canopy height and the vertical (mis)match.}, language = {en} }