Real Microgravity Influences the Cytoskeleton and Focal Adhesions in Human Breast Cancer Cells

With the increasing number of spaceflights, it is crucial to understand the changes occurring in human cells exposed to real microgravity (r-µg) conditions. We tested the effect of r-µg on MCF-7 breast cancer cells with the objective to investigate cytoskeletal alterations and early changes in the gene expression of factors belonging to the cytoskeleton, extracellular matrix, focal adhesion, and cytokines. In the Technische Experimente unter Schwerelosigkeit (TEXUS) 54 rocket mission, we had the opportunity to conduct our experiment during 6 min of r-µg and focused on cytoskeletal alterations of MCF-7 breast cancer cells expressing the Lifeact-GFP marker protein for the visualization of F-actin as well as the mCherry-tubulin fusion protein using the Fluorescence Microscopy Analysis System (FLUMIAS) for fast live-cell imaging under r-µg. Moreover, in a second mission we investigated changes in RNA transcription and morphology in breast cancer cells exposed to parabolic flight (PF) maneuvers (31st Deutsches Zentrum für Luft- und Raumfahrt (DLR) PF campaign). The MCF-7 cells showed a rearrangement of the F-actin and tubulin with holes, accumulations in the tubulin network, and the appearance of filopodia- and lamellipodia-like structures in the F-actin cytoskeleton shortly after the beginning of the r-µg period. PF maneuvers induced an early up-regulation of KRT8, RDX, TIMP1, CXCL8 mRNAs, and a down-regulation of VCL after the first parabola. E-cadherin protein was significantly reduced and is involved in cell adhesion processes, and plays a significant role in tumorigenesis. Changes in the E-cadherin protein synthesis can lead to tumor progression. Pathway analyses indicate that VCL protein has an activating effect on CDH1. In conclusion, live-cell imaging visualized similar changes as those occurring in thyroid cancer cells in r-µg. This result indicates the presence of a common mechanism of gravity perception and sensation.


Introduction
Cancer is a burden of mankind with a high morbidity and mortality and is responsible for an estimated 9.6 million deaths, according to the World Health Organization (WHO) Global Cancer Observatory (GLOBOCAN) data indicated in 2018 [1]. The GLOBOCAN statistics from 2018 published that breast cancer is the most common cancer in women and the second leading cause of cancer deaths worldwide [1]. More women are diagnosed with breast cancer in 2019 than with any other cancer, besides skin cancer. In 2019, an estimated 268,600 women in the United States will be diagnosed with invasive breast cancer, and 62,930 women with in situ breast cancer [2]. In addition, an estimated 2670 men in the United States will be diagnosed with breast cancer.
Due to the high mortality, new ways must be taken to find new approaches and therapeutic strategies in cancer research. Experiments performed in the space environment are not typically the main topic of cancer researchers [3]. However, a stay in orbit on the International Space Station (ISS) provides physical conditions that are not achievable on Earth. Studying the mechanisms of microgravity-dependent cellular and molecular changes is necessary to improve space medicine and to develop new treatment strategies for cancer patients [4].
Gravity is the most familiar force in human life [5]. In space, the gravity force is lowered, resulting in microgravity (µg). Although human cells do not have a gravity sensor, they can still sense µg through the cytoskeleton [6]. The response of cells to early µg, together with changes in actin and microtubules, has been reported for different kinds of cells [7][8][9][10]. Moreover, human thyroid cancer cells have demonstrated a response to early µg by alterations in the cytoskeleton such as disturbance of F-Actin bundles, formation of lamellipodia-and filopodia-like structures and cellular detachment [11]. When cells are subjected to µg for a longer duration, they tend to form three-dimensional (3D) aggregates, so-called multicellular spheroids (MCS) [12].
There are several options to study cells real microgravity (r-µg), such as parabolic flights, sounding rockets missions, unmanned BION and photon spaceflights or a spaceflight in orbit or to the ISS with a commercial carrier. The Technische Experimente unter Schwerelosigkeit (TEXUS, TX) sounding rocket program, offered by the Deutsches Zentrum für Luft-und Raumfahrt (DLR, German Aerospace Center), offers researchers six minutes of µg to conduct their experiments [11,13,14]. We participated in the TX54 mission with the main objective of study cytoskeletal alterations of breast cancer cells in r-µg. Moreover, we attended the 31st DLR parabolic flight campaign (PFC) and investigated morphological changes and focused on the gene expression of selected genes of interest. The Michigan cancer foundation (MCF)-7 cell line was chosen as a suitable candidate for both the TX 54 mission and the PFC. As an alternative to conducting experiment in r-µg, which often is very expensive and time consuming, researchers may choose to investigate biological processes in simulated µg. The simulation of µg is achievable by using the rotating wall vessel (RWV), the random positioning machine (RPM), a 2D or 3D clinostat, and magnetic levitation [15]. These special conditions had been applied to study changes in cell growth and the function of different benign cell types and cancer cells, and may to some extent resemble the findings provided by r-µg [16].
The MCF-7 cell line had been investigated for several times under altered µg conditions in space and on Earth. The MCF-7 cell line showed a robust behavior in µg, and MCF-7 cells had been tested in space in a Photon capsule [17]. The MCF-7 cells reacted by exhibiting alterations in microtubules [17]. In addition, the MCF-7 cells exerted a loosening of the perinuclear cytokeratin network [18]. RPM-exposure experiments of the MCF-7 cells revealed changes in their growth behavior.
In this paper, we report for the first-time live-cell imaging of breast cancer cells on board a sounding rocket (TX 54). Live-cell imaging was performed with a spinning-disc Fluorescence Microscopy Analysis System (FLUMIAS) [11]. The objective of this study was first to focus on changes in the microtubule and F-actin cytoskeleton. Second, we investigated the changes in expression, distribution and localization of selected proteins by indirect immunofluorescence of fixed cells during µg. Third, we examined MCF-7 cells exposed to PF maneuvers and addressed changes in the gene expression patterns of genes encoding for components of the cytoskeleton, the extracellular matrix (ECM), focal adhesion molecules and cytokines.

Results
The TEXUS program is an established DLR-sponsored sounding rocket program which offers researchers precious µg time to test their hypotheses [19]. The sounding rocket has the advantage of providing a relatively longer time (6 min) period of r-µg compared to the parabolic flights. Moreover, it has only one period of hypergravity (hyper-g) and vibration at the beginning prior to the r-µg phase.
The cytoskeleton is a highly dynamic structure playing a crucial role in adaptation and cell signaling processes in µg. We first examined human MCF-7 breast cancer cells on a sounding rocket and studied the early cytoskeletal alterations (F-actin, α-tubulin).
MCF-7 cells exhibited three forms of growth when cultured for 24 days and five days under sµg conditions. One part grew adherently on the cell culture flask bottom, a second group formed duct-like multicellular spheroids and a third group revealed compact spheroids on the RPM after a five-day exposure, whereas after 24h only adherent cells and compact MCS were visible [20,21]. The MCF-7 cells were transfected with a Sleeping Beauty transposon-based (pSB-LAGICT) expression construct to visualize F-actin and α-tubulin. The LAGICT (LifeAct-eGFP-IRES-mCherry-Tubulin) expression cassette enables simultaneous examination of F-actin and α-tubulin, through coexpression of Lifeact GFP and mCherry-tubulin fusion proteins, respectively. Transfected MCF-7 cells were examined with the FLUMIAS microscope with 488 nm and 568 nm diode lasers prior to launch and during r-µg. All the images taken at r-µg were compared to control images ( Figure 1) which were taken before launch. We showed that MCF-7 cells respond to r-µg within four minutes and demonstrate similar changes as the FTC-133 thyroid cancer cells studied in previous campaigns [11]. This indicates a general gravitational mechanism in human cancer cells. During the r-µg phase of the TEXUS flight, various changes in the cytoskeleton were seen, including a clear influence on the F-actin bundles and the appearance of filopodia/lamellipodia-like structures ( Figure 1). . The MCF-7 breast cancer cells 5 min before launch (T-300 s) of the rocket and during the r-µg phase (T + 177s-T + 402s). The yellow arrows show the changes in F-actin (a-e; green fluorescence). The yellow circles include an area with F-actin accumulations. Filopodia and lamellipodia are found after 150s, which are more pronounced with time. The green arrows indicate changes in α-tubulin (f-j; red fluorescence). The tubulin network reveals holes after 150s and a looser structure. . The MCF-7 breast cancer cells 5 min before launch (T-300 s) of the rocket and during the r-µg phase (T + 177s-T + 402s). The yellow arrows show the changes in F-actin (a-e; green fluorescence). The yellow circles include an area with F-actin accumulations. Filopodia and lamellipodia are found after 150s, which are more pronounced with time. The green arrows indicate changes in α-tubulin (f-j; red fluorescence). The tubulin network reveals holes after 150s and a looser structure.

Immunostaining of MCF 7 Cells Exposed to r-µg during the TEXUS 54 Sounding Rocket Mission and Fixed in Orbit
In addition to the live-cell imaging studies of the transfected MCF-7 cells, regular MCF-7 cells were seeded into 18-well Ibidi slides which were fixed with 4% PFA at the end of the µg period and the hyper-g period. These slides were compared to a control slide fixed with 4% PFA on ground. Thus, we had the opportunity to investigate the changes in expression and distribution of the designated proteins. We tested the antibodies MMP9, VEGFA (c-term), IL-6 and IL-8. Phalloidin rhodamine and DAPI stains were used additionally for all the slides from the TX 54 mission.
Upon visual inspection of the microscopic images, there was no apparent difference in the protein distribution between the different conditions for all the tested antibodies (Figure 2a-l). In order to provide an indication on whether the level of the visualized proteins may have changed, the microscopic images were analyzed at the end of the hyper-g and µg phases in comparison to the controls by using the ImageJ program. At the end of the hyper-g phase, the analysis indicated that the level of F-actin was increased (Figure 2c

Immunostaining of MCF 7 cells exposed to r-µg during the TEXUS 54 sounding rocket mission and fixed in orbit
In addition to the live-cell imaging studies of the transfected MCF-7 cells, regular MCF-7 cells were seeded into 18-well Ibidi slides which were fixed with 4% PFA at the end of the µg period and the hyper-g period. These slides were compared to a control slide fixed with 4% PFA on ground. Thus, we had the opportunity to investigate the changes in expression and distribution of the designated proteins. We tested the antibodies MMP9, VEGFA (c-term), IL-6 and IL-8. Phalloidin rhodamine and DAPI stains were used additionally for all the slides from the TX 54 mission.
Upon visual inspection of the microscopic images, there was no apparent difference in the protein distribution between the different conditions for all the tested antibodies (Figure 2a-l). In order to provide an indication on whether the level of the visualized proteins may have changed, the microscopic images were analyzed at the end of the hyper-g and µg phases in comparison to the controls by using the ImageJ program. At the end of the hyper-g phase, the analysis indicated that the level of F-actin was increased (Figure 2c  Indirect immunofluorescence staining of PFA-fixed cells from the TEXUS 54 sounding rocket mission. 2500 MCF-7 cells were seeded into each well of the 18 well Ibidi slides. The cells were fixed either at the end of the hyper-g period or at the end of the µg period. The two conditions were compared to 1g-ground control samples. The confocal laser scanning microscopy images (a-l) show either MMP9, VEGF-A, IL-6 or IL-8 in green, DAPI (in blue) and F-Actin (in red). Scale bar is equal to 50 µm. The intensity of the staining was quantified by ImageJ (m-q). All data are shown as mean ± SD, n = 10-14, with significance indicated by * p < 0.05.

Results of the 31 st DLR Parabolic Flight Campaign: "Effects Of Short-Term Microgravity on Human Breast Cancer Cells"
The PFCs were organized by the DLR in close collaboration with the company Novespace, Bordeaux-Mérignac, France. A parabolic flight consisted of 31 consecutive parabolas. Each parabola contains two phases of 1.8 g hyper-g spanning one phase of 10 −2 g r-µg. The first phase of a parabola begins with flying at 45 degrees for 22 s known as pull-up, followed by decreasing thrust and following the trajectory of a parabola for 22 s of free-fall. Thus, the r-µg phase lasts for the 22 s of the free-fall. The last phase is known as pull-out which begins pulling out the plane to fly back on a horizontal line trajectory. The pull-up phase lasts for 22 s with hyper-g of 1.8 g [16,22,23]. Not only does the parabolic flight have the advantage of offering valuable r-µg time to researchers, but also it gives the scientists access to their experiment on board of the flight.
The 31 st DLR PFC took place in March 2018 at the company Novespace at the Bordeaux-Mérignac airport in France. The breast cancer cells (MCF-7 cell line) were examined after parabola 1 (P1) and after 31 parabolas (P31). At the same time, the ground control experimentation took place in the laboratories of Novespace. Subsequently, the fixed cells were transported to the Otto von Guericke University Magdeburg, Germany, where they were examined by molecular biology. We performed qPCR, Western blot and pathway analyses. The results are shown in the following Figures 3-10.   Figure 4 shows the levels of the corresponding proteins. There were no changes after P1 for the ACTB, TUBB, EZR, RDX and MSN mRNAs. However, there was a significant up-regulation of KRT8 after P1 and P31 compared to 1g ( Figure 3c) and of RDX after P31 (Figure 3e). The cytokeratin protein synthesis was also significantly increased after the first parabola but returned to control levels after 31 parabolas (Figure 4c). Indirect immunofluorescence staining of PFA-fixed cells from the TEXUS 54 sounding rocket mission. 2500 MCF-7 cells were seeded into each well of the 18 well Ibidi slides. The cells were fixed either at the end of the hyper-g period or at the end of the µg period. The two conditions were compared to 1g-ground control samples. The confocal laser scanning microscopy images (a-l) show either MMP9, VEGF-A, IL-6 or IL-8 in green, DAPI (in blue) and F-Actin (in red). Scale bar is equal to 50 µm. The intensity of the staining was quantified by ImageJ (m-q). All data are shown as mean ± SD, n = 10-14, with significance indicated by * p < 0.05.

Results of the 31st DLR Parabolic Flight Campaign: "Effects Of Short-Term Microgravity on Human Breast Cancer Cells"
The PFCs were organized by the DLR in close collaboration with the company Novespace, Bordeaux-Mérignac, France. A parabolic flight consisted of 31 consecutive parabolas. Each parabola contains two phases of 1.8 g hyper-g spanning one phase of 10 −2 g r-µg. The first phase of a parabola begins with flying at 45 degrees for 22 s known as pull-up, followed by decreasing thrust and following the trajectory of a parabola for 22 s of free-fall. Thus, the r-µg phase lasts for the 22 s of the free-fall. The last phase is known as pull-out which begins pulling out the plane to fly back on a horizontal line trajectory. The pull-up phase lasts for 22 s with hyper-g of 1.8 g [16,22,23]. Not only does the parabolic flight have the advantage of offering valuable r-µg time to researchers, but also it gives the scientists access to their experiment on board of the flight.
The 31st DLR PFC took place in March 2018 at the company Novespace at the Bordeaux-Mérignac airport in France. The breast cancer cells (MCF-7 cell line) were examined after parabola 1 (P1) and after 31 parabolas (P31). At the same time, the ground control experimentation took place in the laboratories of Novespace. Subsequently, the fixed cells were transported to the Otto von Guericke University Magdeburg, Germany, where they were examined by molecular biology. We performed qPCR, Western blot and pathway analyses. The results are shown in the following   Figure 4 shows the levels of the corresponding proteins. There were no changes after P1 for the ACTB, TUBB, EZR, RDX and MSN mRNAs. However, there was a significant up-regulation of KRT8 after P1 and P31 compared to 1g ( Figure 3c) and of RDX after P31 (Figure 3e). The cytokeratin protein synthesis was also significantly increased after the first parabola but returned to control levels after 31 parabolas (Figure 4c).   The data are given as mean ± standard deviation. * p < 0.05 vs. Control; # p < 0.05 vs. P1.

Altered Expression of Genes of the Focal Adhesion Complex
Furthermore, we examined the mRNA expression and protein content of focal adhesion molecules ( Figures 5 and 6). The VCL gene and corresponding vinculin protein were significantly reduced under r-µg (Figures 5a and 6a). TLN1, ITGB1, CDH1, PTK2, CAV1 and CAV2 remained unchanged under r-µg, while the E-cadherin protein (Figure 6c) as well as β1-integrin protein ( Figure  6b) were significantly reduced. FAK1 protein was elevated after P1 ( Figure 6d).   The data are given as mean ± standard deviation. * p < 0.05 vs. Control; # p < 0.05 vs. P1.

Altered Expression of Genes of the Focal Adhesion Complex
Furthermore, we examined the mRNA expression and protein content of focal adhesion molecules ( Figures 5 and 6). The VCL gene and corresponding vinculin protein were significantly reduced under r-µg (Figures 5a and 6a). TLN1, ITGB1, CDH1, PTK2, CAV1 and CAV2 remained unchanged under r-µg, while the E-cadherin protein ( Figure 6c) as well as β1-integrin protein ( Figure  6b) were significantly reduced. FAK1 protein was elevated after P1 ( Figure 6d).

Altered Expression of Genes of the Focal Adhesion Complex
Furthermore, we examined the mRNA expression and protein content of focal adhesion molecules ( Figures 5 and 6). The VCL gene and corresponding vinculin protein were significantly reduced under r-µg (Figures 5a and 6a). TLN1, ITGB1, CDH1, PTK2, CAV1 and CAV2 remained unchanged under r-µg, while the E-cadherin protein ( Figure 6c) as well as β 1 -integrin protein ( Figure 6b) were significantly reduced. FAK1 protein was elevated after P1 ( Figure 6d).

Figure 5.
Influence of short-term microgravity on the expression (mRNA) of focal adhesion complex components. The data is given as mean ± standard deviation. * p < 0.05 vs. Control. Figure 6. Influence of short-term microgravity on the protein accumulation of focal adhesion complex components. The data is given as mean ± standard deviation. * p < 0.05 vs. Control.

Changes of Extracellular Matrix and Cytokine Gene Expression
The results on the extracellular matrix proteins are shown in Figures 7 and 8. There were no changes in the gene expression for LAMA1, LAMA3, COL1A1, FN1, MMP9 and PAI1 (SERPINE1). The TIMP1 mRNA was significantly elevated after P31 compared with ground control samples ( Figure 7e). In addition, we investigated the expression of the cytokines IL-6 and IL-8, which play a major role in spheroid formation. The IL6 mRNA was not significantly changed, but there was a Figure 5. Influence of short-term microgravity on the expression (mRNA) of focal adhesion complex components. The data is given as mean ± standard deviation. * p < 0.05 vs. Control. Figure 5. Influence of short-term microgravity on the expression (mRNA) of focal adhesion complex components. The data is given as mean ± standard deviation. * p < 0.05 vs. Control. Figure 6. Influence of short-term microgravity on the protein accumulation of focal adhesion complex components. The data is given as mean ± standard deviation. * p < 0.05 vs. Control.

Changes of Extracellular Matrix and Cytokine Gene Expression
The results on the extracellular matrix proteins are shown in Figures 7 and 8. There were no changes in the gene expression for LAMA1, LAMA3, COL1A1, FN1, MMP9 and PAI1 (SERPINE1). The TIMP1 mRNA was significantly elevated after P31 compared with ground control samples ( Figure 7e). In addition, we investigated the expression of the cytokines IL-6 and IL-8, which play a major role in spheroid formation. The IL6 mRNA was not significantly changed, but there was a Figure 6. Influence of short-term microgravity on the protein accumulation of focal adhesion complex components. The data is given as mean ± standard deviation. * p < 0.05 vs. Control.

Changes of Extracellular Matrix and Cytokine Gene Expression
The results on the extracellular matrix proteins are shown in Figures 7 and 8. There were no changes in the gene expression for LAMA1, LAMA3, COL1A1, FN1, MMP9 and PAI1 (SERPINE1). The TIMP1 mRNA was significantly elevated after P31 compared with ground control samples ( Figure 7e). In addition, we investigated the expression of the cytokines IL-6 and IL-8, which play a major role in spheroid formation. The IL6 mRNA was not significantly changed, but there was a tendency of an up-regulation after P1 and P31 (Figure 7h). In contrast, CXCL8 was significantly up-regulated after P1, and slightly elevated after P31 (Figure 7i). A similar behavior showed the corresponding IL-8 protein synthesis, which was significantly increased after P1 and P31 ( Figure 8). Moreover, a significant elevation of the VEGFA mRNA was detectable (Figure 7j). tendency of an up-regulation after P1 and P31 ( Figure 7h). In contrast, CXCL8 was significantly upregulated after P1, and slightly elevated after P31 (Figure 7i). A similar behavior showed the corresponding IL-8 protein synthesis, which was significantly increased after P1 and P31 ( Figure 8). Moreover, a significant elevation of the VEGFA mRNA was detectable ( Figure 7j).   tendency of an up-regulation after P1 and P31 ( Figure 7h). In contrast, CXCL8 was significantly upregulated after P1, and slightly elevated after P31 (Figure 7i). A similar behavior showed the corresponding IL-8 protein synthesis, which was significantly increased after P1 and P31 ( Figure 8). Moreover, a significant elevation of the VEGFA mRNA was detectable ( Figure 7j).

Figure 8.
Influence of short-term microgravity on the protein accumulation of IL-8. The data is given as mean ± standard deviation. * p < 0.05 vs. Control. Figure 8. Influence of short-term microgravity on the protein accumulation of IL-8. The data is given as mean ± standard deviation. * p < 0.05 vs. Control.

Pathway Analyses
The results of the pathway analysis given in Figure 9 indicate a clear role for ITGB1, FN1, TLN1, CDH1, PTK2 and VCL in gravity sensing of MCF-7 breast cancer cells exposed to short-term r-µg.
FN1, VEGFA, TLN1 and TIMP1 proteins are positively influencing β 1 -integrin which is inducing PTK2 and fibronectin. TLN1 is interacting with PTK2 and FN1. Vinculin is activating E-cadherin, whereas ezrin has a negative influence on CDH1. Moreover, TIMP1 is inhibiting MMP9. The results of the pathway analysis given in Figure 9 indicate a clear role for ITGB1, FN1, TLN1, CDH1, PTK2 and VCL in gravity sensing of MCF-7 breast cancer cells exposed to short-term r-µg.   The results of the pathway analysis given in Figure 9 indicate a clear role for ITGB1, FN1, TLN1, CDH1, PTK2 and VCL in gravity sensing of MCF-7 breast cancer cells exposed to short-term r-µg.   The interaction network shown in Figure 10 indicates a fast significant up-regulation of KRT8, RDX, TIMP1 and CXCL8, while VCL is down-regulated. Simultaneously, TLN1 and CDH1 indicate a slight but non-significant reduction of gene expression. Considering the red lines together with the qPCR results cell adhesion via CDH1 seems to be attenuated. Various genes demonstrate an inhibitory effect on CDH1 (Figure 9).

Discussion
In this study we investigated MCF-7 breast cancer cells in real microgravity using two experimental platforms offered by a sounding rocket mission and a parabolic flight. Live-cell imaging visualized similar changes as those occurring in thyroid cancer cells, when they were exposed to r-µg. Our results now indicate the presence of a common cellular mechanism for sensing gravity. After entering microgravity, the MCF-7 cells showed a rearrangement of F-actin and tubulin comprising holes, accumulations in the tubulin network, and the appearance of filopodia-and lamellipodia-like structures. Up-regulation of VEGF and down-regulation of E-cadherin during parabolic flight maneuvers indicated a temporary change to a more invasive phenotype of MCF-7 cells. This finding also supports earlier data gained from thyroid cancer cells and may hint at a general cellular answer of cancer cells to short-term microgravity.
There is evidence that in vitro cell cultures respond to altered gravity conditions. Studies suggest that this response might be involved in the physiological changes and fundamental health problems of humans during spaceflight [24]. Microgravity alters adhesion, migration, proliferation, differentiation, growth, signaling and gene expression [25]. The cytoskeleton is discussed as the initial gravity sensor [26]. For example, bone cells exposed to r-and s-µg show changes in their cytoskeleton and focal adhesions, two major mechanosensitive structures [27,28]. Similar results were obtained when investigating thyroid cancer and melanoma cells cultured under µg-conditions [14,29].
Live-cell imaging of benign and tumor cells is possible using the FLUMIAS microscope which was flown on parabolic flight missions, sounding rocket missions and a more advanced version to the ISS [11,30].

Cytoskeletal Alterations Visualized during the TEXUS 54 Mission
The principal aim of our experiment onboard the TX 54 sounding rocket was to investigate the effect of r-µg on the cytoskeleton of human breast cancer cells.
During the flight, MCF-7 cells exhibited alterations in the F-actin and microtubule cytoskeleton. The appearance of filopodia-and lamellipodia-like structures shortly after the beginning of the r-µg period is comparable to the results which we have obtained with FTC-133 thyroid cancer cells during the TX 52 mission [11]. This data indicates that the gravi-sensing is similar in both cancer types. We could visualize impressing changes of alpha-tubulin during the r-µg phase. This supports earlier results [20]. Investigating suspensions of purified tubulin, Moos et al. [31] found a significant difference between microtubules assembled in the 30 s µg phase and the 2g hyper-g phase of a PF. These data reveal that microtubule polymerization is altered by altered gravity. These results were substantiated by sounding rocket [32] and shuttle flight [33] experiments.
In addition, an immunofluorescence staining on MCF-7 cells was performed. The cell fixation was done automatically during the r-µg phase of the TX 54 mission. The quantitative analysis of VEGF exhibited an up-regulation of the protein in the r-µg condition compared to the controls. We also measured an accumulation of F-actin. While VEGFA was up-regulated only in the r-µg condition, F-actin was increased in both the hyper-g and r-µg conditions. The significant up-regulation of a protein in both µg and hyper-g conditions indicates that hyper-g was the main inducer for the up-regulation, because the hyper-g period precedes the µg period. The F-actin content was elevated in A431 epidermoid carcinoma cells after a 7-min µg-exposure during a sounding rocket flight [34]. Boonstra concluded that the actin microfilament system is sensitive to altered gravity conditions and that its remodeling may affect signal transduction [34]. Reflecting our results, we can support this hypothesis.
Therefore, we can conclude that only VEGF showed a clear up-regulation in r-µg compared to the control. This data fits to earlier results obtained during a PF mission, where VEGF was significantly up-regulated after P1 and P31 [16]. VEGF is a key inducer of angiogenesis and enhances spreading and metastasis [35,36]. Serum VEGF was significantly elevated in patients with metastatic differentiated thyroid cancer but not in those with poorly differentiated thyroid cancer metastases [37]. The release of VEGF by FTC-133 exposed to space conditions during the Shenzhou-8 spaceflight was high but not significantly different in 1g samples and r-µg samples, but the gene expression of VEGFA was down-regulated after a 10-day mission [16].

MCF-7 Breast Cancer Cells Exposed to PF Maneuvers during the 31st DLR PFC
Earlier experiments investigating chondrocytes, endothelial cells, and thyroid cancer cells revealed that a short-term r-µg-exposure (22 s) during PF maneuvers induced early cytoskeletal changes and an altered gene expression pattern in these different cell types [22,38,39]. These studies showed that the gravi-response of cancer and benign cells occurred very early, within the first few seconds [22,38,39]. Several gravi-sensitive signaling elements, such as AMP-activated protein kinase alpha 1 and integrins are involved in the reaction of endothelial cells to altered gravity conditions [38]. Down-regulated MTSS1 and up-regulated LIMA1 were key factors stabilizing the cytoskeleton of tumor cells under µg conditions [39].
ECM proteins, focal adhesion and cytoskeletal components form a dynamic network interacting with signaling molecules as an adaptive response to altered gravity. These focal adhesions are integrin-containing structures that form mechanical links between intracellular actin bundles and the extracellular space of a cell. Focal adhesions are dynamic protein complexes through which the cytoskeleton of a cell connects to the ECM. The adhesion dynamics play a central role in cellular migration. Focal complexes are formed at the leading edge of the cell in lamellipodia.
We had first investigated the gene expression of cytoskeletal factors. Most cytoskeletal genes were not significantly altered but there was a significant up-regulation of the KRT8 mRNA after P1 and P31. This finding is similar to earlier results with thyroid cancer cells [39].
Studying the genes of the focal adhesion complex we found a decrease in E-cadherin protein as well as β 1 -integrin protein. Changes in the focal adhesion complex were also found in cells exposed to s-µg and r-µg. Tan et al. [29] reported about a reduction in focal adhesions in melanoma cells exposed to s-µg. In space on board the SJ-10 satellite, the mechanosensitive molecules β 1 -integrin, β-actin, α-tubulin, and others were elevated, whereas among others vinculin was down-regulated in bone marrow-derived mesenchymal stem cells [40]. In addition, the authors observed an accumulation of microtubules and vimentin through the altered expression and location of focal adhesion complexes [40].
Several ECM genes such as FN1 were not altered during short-term µg in MCF-7 breast cancer cells. This is different to the results which we obtained from low-differentiated ML-1 thyroid cancer cells [39]. During this PFC we detected an up-regulation of the FN1 mRNA, which indicates a cancer type-specific reaction to µg. β 1 -integrin, fibronectin, and PTK2 play essential roles, when cells bind to the extracellular matrix. β 1 -integrin is involved in the proliferation and differentiation as well as in the development of epithelial tissues [41]. It is important for adhesion dynamics and essential for the control of cell migration and, therefore, is a marker for a poor prognosis in breast cancer [41]. β 1 -integrin forms heterodimers with various α-types integrins. Some of these dimers are able to bind to fibronectin. After binding, signals are forwarded to FAK1 (Focal adhesion kinase 1 coded by PTK2) and talin (TLN1) [42].
Binding of β 1 -integrin to fibrillar fibronectin promotes the phosphorylation of STAT3, which is known to participate in the induction of the epithelial mesenchymal transition [43]. In addition, β 1 -integrin facilitates the secretion of fibronectin in a way which is poorly understood. Fibronectin remaining intracellular is directly interacting with the actin cytoskeleton [43], which is changed when the cells are exposed to microgravity [20]. Moreover, β 1 -integrin controls the VE-cadherin localization and blood vessel stability in the mouse retina [44]. VEGF can promote angiogenesis through up-regulation and/or activation of integrins [45]. The VEGF activity is dependent on β 1 -integrin function.
FAK1 and talin are members of the focal adhesion complexes. Talin mediates cell-cell adhesion linking the integrins to the actin cytoskeleton and in the activation of integrins [46]. Talin was differentially regulated in AD and MCS of thyroid cancer cells exposed to simulated microgravity [47]. FAK1 is a cytoplasmic protein tyrosine, kinase which is found to be concentrated in the focal adhesions. It promotes the organization of the fibronectin matrix and fibrillar adhesions [48]. In addition, FAK1 triggers the recruitment of talin to nascent adhesions independently of integrin. It plays a key role in the migration process and FAK1 inhibition decreases mobility and metastasis. The β1-Integrin-FAK pathway is involved in cell survival and on the role of FAK in breast cancer development and progression [49]. In this study, the PTK2 mRNA was stable in the breast cancer cells, but the corresponding protein showed an elevation after P1 (Figure 6d). This is different to the data obtained with thyroid cancer cells, where the PTK2 mRNA in FTC-133 thyroid cancer cells was differentially expressed in the TEXUS samples, but the FAK1 protein content was significantly reduced in RPM samples [14].
The pathway analysis of the investigated genes revealed important roles of CDH1 and VEGFA in the network. These genes are under the influence of IL-6 and IL-8, which both exert inhibitory effects on CDH1 and promoting effects on VEGFA. IL-6 promotes e-cadherin repression [50] and treating human gastric carcinoma cells with exogenous IL-8 decreased expression of E-cadherin mRNA [51]. IL-6 and IL-8 induce the expression of VEGF [52,53]. The CDH1 gene encodes e-cadherin, which establishes cell-cell junctions [54]. After a 2-week RPM-exposure, E-cadherin, was diminished in MCF-7 MCS cells, where proteins of the E-cadherin autodegradation pathway were enhanced as well as c-Src (proto-oncogene tyrosine-protein kinase c-Src) [55]. Blocking the E-cadherin activity by specific antibodies promoted spheroid formation. As indicated by the high number of red lines shown in Figure 10, CDH1 gene expression is strongly controlled by a number of proteins. Of the investigated components, only vinculin has a positive modulatory influence (green arrow) [56].
But, in addition to IL-6 and IL-8, EZR, talin, PTK2, ITGB1 and MMP9 were already found to have inhibitory effects. E-cadherin and EZR are involved in tumor growth. In a patient study, the ezrin expression was upregulated, while that of E-cadherin was decreased in breast cancer as compared to the control specimen. Ezrin expression was negatively correlated to the E-cadherin expression in a subpopulation of breast cancer patients with a high expression of ezrin [ezrin(high)] and a low expression of E-cadherin [E-cad(low)] [57]. Talin regulates the stability of E-cadherin transcriptional repressors [58]. An increased expression of E-cadherin was observed after reducing the level of β 1 -integrin in B16-F10 melanoma cells [59]. Treatment with recombinant MMP-9 or transient expression of MMP-9 is sufficient to reduce E-cadherin levels in differentiated ovarian tumor cells [60].
VEGFA encodes the vascular endothelial growth factor, which supports (neo)-vascularization of healthy and malignant tissues [61]. As mentioned above, IL-6 and IL-8 favor its expression. In addition, human astrocytoma cells expressed increased levels of fibronectin and VEGF upon transformation with a versican G3 construct [62] and VEGF expression was positively linked to MMP-9 levels in gastric carcinoma [63]. Overexpression of TIMP1 and PAI-1 in endothelial cells blocks vascular tube regression [64].

Microgravity-Induced Cytoskeleton Changes and Potent Physiological Responses
The cytoskeleton directs a number of essential cell functions, such as maintenance of cell shape, support of vacuole formation or fixation of organelles. The cytoskeleton is dynamic and not static, and it can disassemble and reassemble to contribute to cell mobility ( Figure 11). It is involved in migration which is necessary for tissue repair and tumor spreading, progression and metastasis [65]. It is important for cellular signaling.
In this study, we demonstrate for the first time using live-cell imaging in real µg that MCF-7 cells reveal a rearrangement of the F-actin and microtubule cytoskeleton with holes, accumulations in the tubulin network, and the appearance of filopodia-and lamellipodia-like structures in the F-actin cytoskeleton (Figure 1). In lamellipodia are ribs of actin called microspikes spreading beyond the lamellipodium frontier are then called filopodia, which are involved in cell adhesion and migration, healing processes and others. The initiation and elongation of filopodia is depending on polymerization, convergence and crosslinking of actin filaments [66]. Filopodia and filopodia-like structures are involved in 3D cell migration and thus in tumor dissemination, growth and metastasis [67]. Filopodia are normally situated at the front of invading cancer cells [68,69] and filopodia-like structures promote cancer cell survival at metastatic sites [70,71]. In Figure 11 the possible mechanism is demonstrated how these µg-induced alterations of the cytoskeleton are involved in 3D growth and in the formation of multicellular spheroids, which resemble in vivo microtumors and metastases [65].  (Figure 1). In lamellipodia are ribs of actin called microspikes spreading beyond the lamellipodium frontier are then called filopodia, which are involved in cell adhesion and migration, healing processes and others. The initiation and elongation of filopodia is depending on polymerization, convergence and crosslinking of actin filaments [66]. Filopodia and filopodia-like structures are involved in 3D cell migration and thus in tumor dissemination, growth and metastasis [67]. Filopodia are normally situated at the front of invading cancer cells [68,69] and filopodia-like structures promote cancer cell survival at metastatic sites [70,71]. In Figure 11 the possible mechanism is demonstrated how these µg-induced alterations of the cytoskeleton are involved in 3D growth and in the formation of multicellular spheroids, which resemble in vivo microtumors and metastases [65]. In this study PF maneuvers induced a downregulation of VCL mRNA and the corresponding protein in MCF-7 breast cancer cells. Pathway analyses indicated that VCL protein has an activating effect on CDH1. E-cadherin is involved in cell adhesion and in tumorigenesis. Changes in the Ecadherin protein synthesis can lead to tumor progression. In addition, blockage of E-cadherin and a down-regulation of CDH1 leads to enhanced spheroid formation of MCF-7 breast cancer cells [55,65].
r-µg-induced changes in the cytoskeleton and/or in focal adhesion components of human cells as for example cancer cells and normal cells like osteoblasts, chondrocytes and cancer cells are the two major mechanosensitive responses [8,14,28]. The cytoskeleton responds to changes in the mechanical environment because of its connection to the ECM through focal adhesions. Exposure of human cells to µg impaired their cytoskeleton stability and reduced cellular tension, as well as focal adhesion formation and stability [8].
The ECM-membrane receptors-cytoskeleton system is known to be involved in cancer and metastasis [72]. Growth factor receptors, adhesion proteins and ion channels in association with the sub-membranous system of the actin cytoskeleton control the actin microfilament's force generating capacity. Perturbations of the actin microfilament system in cell motility and migration and their role in cancer pathophysiology are currently a hot topic [72].
The exact mechanisms how the cells transform the mechanical signal (microgravity) into a biochemical signal is still not known. The widely acknowledged tensegrity model hypothesis proposed by Ingber [73] explains that the cells are hardwired by the cytoskeleton components. The cells are spanned open and are under continuous tension [26,73]. An imbalance between adhesion Figure 11. Alterations of adherently growing cancer cells after exposure to microgravity (modified from [65]). The figure in the box shows changes at the microscopic level. F-actin is displayed as green lines, the ECM in yellow. FP: filopodia, LP: lamellipodia.
In this study PF maneuvers induced a downregulation of VCL mRNA and the corresponding protein in MCF-7 breast cancer cells. Pathway analyses indicated that VCL protein has an activating effect on CDH1. E-cadherin is involved in cell adhesion and in tumorigenesis. Changes in the E-cadherin protein synthesis can lead to tumor progression. In addition, blockage of E-cadherin and a down-regulation of CDH1 leads to enhanced spheroid formation of MCF-7 breast cancer cells [55,65].
r-µg-induced changes in the cytoskeleton and/or in focal adhesion components of human cells as for example cancer cells and normal cells like osteoblasts, chondrocytes and cancer cells are the two major mechanosensitive responses [8,14,28]. The cytoskeleton responds to changes in the mechanical environment because of its connection to the ECM through focal adhesions. Exposure of human cells to µg impaired their cytoskeleton stability and reduced cellular tension, as well as focal adhesion formation and stability [8].
The ECM-membrane receptors-cytoskeleton system is known to be involved in cancer and metastasis [72]. Growth factor receptors, adhesion proteins and ion channels in association with the sub-membranous system of the actin cytoskeleton control the actin microfilament's force generating capacity. Perturbations of the actin microfilament system in cell motility and migration and their role in cancer pathophysiology are currently a hot topic [72].
The exact mechanisms how the cells transform the mechanical signal (microgravity) into a biochemical signal is still not known. The widely acknowledged tensegrity model hypothesis proposed by Ingber [73] explains that the cells are hardwired by the cytoskeleton components. The cells are spanned open and are under continuous tension [26,73]. An imbalance between adhesion and the cytoskeleton network might induce a cell shape change and has a direct impact on cell signaling [26,73]. This theory is supported by data of cytoskeletal changes in various benign and malignant cell types after short-term exposure to microgravity [11,16,21,22,38,74].
When microgravity conditions influence human adherent MCF-7 breast cancer cells, the microtubules (tubulin) rapidly reorient themselves and actin stress fibers increase in density in order to reinforce their mechanical strength. These changes in the F-actin and in microtubule network are followed by changes in adhesion, shedding of membrane receptors, cell detachment, migration, growth behavior, differentiation, and apoptosis [12,20,38,75]. These physiological changes have been detected in real microgravity and on Earth using various µg-simulation devices [15].
In summary, an early up-regulation of KRT8, RDX, TIMP1, CXCL8, and down-regulation of VCL were found after the PF maneuvers. E-cadherin protein was reduced after the PF maneuvers. This result is very important because E-cadherin is not only involved in the cell adhesion process but plays a significant role in tumorigenesis. Changes in the E-cadherin protein can lead to tumor progression. VCL protein has an activating effect on CDH1 (Figure 9). However, many of the genes investigated lead to an inhibition of CDH1 ( Figure 10). CXCL8 is also important for tumor progression and the early up-regulation of the cytokine supports this thesis.

Cell Culture
The MCF-7 breast cancer cells were purchased from the American Type Culture Collection (MCF7, ATCC ® HTB-22™). They were cultured in RPMI 1640 (Life Technologies, Paisley, UK), 10 % FCS (Sigma Aldrich, Steinheim, Germany) and 1% penicillin/ streptomycin (Life Technologies, New York, NY, USA). The Lifeact-eGFP-IRES-mCherry-Tubulin MCF-7 expressing cells were cultured in the same medium, in addition to G418 (Geneticin) to allow the growth of the stably transfected cells. The cells were cultured in T-75 flasks and the cells were harvested and seeded into other flasks every 3-5 days to prevent confluence.

Construction of An Expression Cassette to Visualize F-actin and α-tubulin
We constructed a pcDNA3.1 LifeAct-eGFP-IRES-mCherry-Tubulin (pLAGICT) expression cassette for visualization of F-acting and α-tubulin. In order to construct this expression cassette, pUC57 plasmid was ordered from GenScript. The required cassette LifeAct-eGFP-IRES-mCherry-Tubulin was excised from the pUC57 plasmid with NotI/XbaI restriction enzymes. The excised part was further purified by gel extraction and ligated into pcDNA3.1 (+) (Invitrogen, Carlsberg, CA, USA). The constructed plasmid was transformed into ultra-competent Escherichia coli cells to produce more copies of the plasmid. QIAprep spin column (Qiagen, Hilden, Germany) was used to extract the plasmid from the bacteria. More details about the construction of the expression cassette are mentioned in [11,76].

Live Cell Imaging by the FLUMIAS Microscope
Approximately 7000 MCF-7 cells were seeded into one channel of an ibiTreat µ-slide VI 0.4 (Ibidi, Gräfelfingen, Germany). The slide was temperature controlled and loaded into the FLUMIAS microscope (developed by FEI Munich GmbH [11]) shortly before the launch (Figure 12). Five minutes prior to launch three z-stacks were obtained from pre-selected cells as a ground control. About 75s after launch the microgravity phase was reached, and the microscope started recording the pre-selected cells. Three z-stacks were taken every one minute with 125 ms exposure time. The thickness of the z-stack was 21 µm with 0.5 µm step size. The procedure was repeated four times with a total number of five active phases covering 6 min of microgravity.
After recovery of the image data, a single image was extracted from each z-stack taken during microgravity to allow analysis of all images in the focal plane. The extracted images were deconvolved by Huygens Essential Scientific Volume Imaging software 4.3 and compared to a control image taken on ground.

TEXUS 54 Sounding Rocket Mission
The late access unit ( Figure 13) was transferred into the payload, along with the cells shortly before launch. The sounding rocket, used in the TEXUS 54 mission, was composed of the payload and a Brazilian two-stage solid propellant VSB 30 rocket. The rocket was launched on the 13th of May 2018 from ESRANGE space center in Kiruna, Sweden. After launch, the sounding rocket reached an altitude of~260 km. And it entered microgravity 75 s later after launch. The microgravity phase of < 10 −4 g lasted for~353 s. Following the microgravity phase, the rocket went back to Earth by a parachute-mediated deceleration. The payload was recovered after landing by a helicopter (Figure 13).

Live Cell Imaging by the FLUMIAS Microscope
Approximately 7000 MCF-7 cells were seeded into one channel of an ibiTreat µ-slide VI 0.4 (Ibidi, Gräfelfingen, Germany). The slide was temperature controlled and loaded into the FLUMIAS microscope (developed by FEI Munich GmbH [11]) shortly before the launch (Figure 12). Five minutes prior to launch three z-stacks were obtained from pre-selected cells as a ground control. About 75s after launch the microgravity phase was reached, and the microscope started recording the pre-selected cells. Three z-stacks were taken every one minute with 125 ms exposure time. The thickness of the z-stack was 21 µm with 0.5 µm step size. The procedure was repeated four times with a total number of five active phases covering 6 min of microgravity.
After recovery of the image data, a single image was extracted from each z-stack taken during microgravity to allow analysis of all images in the focal plane. The extracted images were deconvolved by Huygens Essential Scientific Volume Imaging software 4.3 and compared to a control image taken on ground.

TEXUS 54 Sounding Rocket Mission
The late access unit ( Figure 13) was transferred into the payload, along with the cells shortly before launch. The sounding rocket, used in the TEXUS 54 mission, was composed of the payload and a Brazilian two-stage solid propellant VSB 30 rocket. The rocket was launched on the 13 th of May 2018 from ESRANGE space center in Kiruna, Sweden. After launch, the sounding rocket reached an altitude of ~260 km. And it entered microgravity 75 s later after launch. The microgravity phase of < 10 −4 g lasted for ~353 s. Following the microgravity phase, the rocket went back to Earth by a parachute-mediated deceleration. The payload was recovered after landing by a helicopter ( Figure  13).

FLUFIX and Immunocytochemistry of MCF-7 Fixed Cells during TEXUS 54
The MCF 7 cells were cultured in 18 well Ibidi slides. Approximately 2500 cells were seeded into each well. 4 slides were cultured on ground at 1g to be used as a control. Furthermore, there were four 18 well Ibidi slides on board of the rocket. The cells, on board of the rocket, were fixed with 4% paraformaldehyde (PFA) at two time points. Two Ibidi slides were fixed at the end of the hyper gravity phase and the other two slides were fixed at the end of the microgravity phase. The ground control slides were fixed with 4% PFA in parallel to the launch of the rocket. The slides were recovered and transferred back to the lab in 4% PFA.
To discard excess PFA, the cells were washed with DPBS three times. Afterwards, the slides were washed with 0.3% Triton X in DPBS for 10 min with agitation which was followed by washing with DPBS. To prevent non-specific binding, the slides were incubated in 3% BSA for one hour. Primary antibodies were added to the slides overnight at 4 °C ( Table 1). The following day, the slides were washed with DPBS and the secondary antibody Alex Fluor 488 anti-mouse/anti-rabbit was added for one hour ( Table 1). The slides were washed again with DPBS and Alexa Fluor 568 phalloidin was added for one hour, followed by washing with DPBS and mounting with Fluoroshield with DAPI (Sigma). For the slides to be ready for examination, they were incubated overnight at 4 °C. Carl ZEISS LSM 800 Confocal laser scanning microscope was used to examine the cells. Three lasers were used to examine the slides: 488 nm, 561 nm and 405 nm for visualization of Alexa 488, Alexa 568 and DAPI, respectively.
The microscopic images were quantitatively analyzed by ImageJ 1.52b (U.S. National Institutes of Health, Bethesda, MD, USA) to detect the difference in protein expression between different conditions. The intensity of the fluorescence in every photo was measured by ImageJ after the areas of interest were defined by the wand (tracing) tool. Furthermore, all the values were normalized to background fluorescence.

FLUFIX and Immunocytochemistry of MCF-7 Fixed Cells during TEXUS 54
The MCF 7 cells were cultured in 18 well Ibidi slides. Approximately 2500 cells were seeded into each well. 4 slides were cultured on ground at 1g to be used as a control. Furthermore, there were four 18 well Ibidi slides on board of the rocket. The cells, on board of the rocket, were fixed with 4% paraformaldehyde (PFA) at two time points. Two Ibidi slides were fixed at the end of the hyper gravity phase and the other two slides were fixed at the end of the microgravity phase. The ground control slides were fixed with 4% PFA in parallel to the launch of the rocket. The slides were recovered and transferred back to the lab in 4% PFA.
To discard excess PFA, the cells were washed with DPBS three times. Afterwards, the slides were washed with 0.3% Triton X in DPBS for 10 min with agitation which was followed by washing with DPBS. To prevent non-specific binding, the slides were incubated in 3% BSA for one hour. Primary antibodies were added to the slides overnight at 4 • C ( Table 1). The following day, the slides were washed with DPBS and the secondary antibody Alex Fluor 488 anti-mouse/anti-rabbit was added for one hour ( Table 1). The slides were washed again with DPBS and Alexa Fluor 568 phalloidin was added for one hour, followed by washing with DPBS and mounting with Fluoroshield with DAPI (Sigma). For the slides to be ready for examination, they were incubated overnight at 4 • C. Carl ZEISS LSM 800 Confocal laser scanning microscope was used to examine the cells. Three lasers were used to examine the slides: 488 nm, 561 nm and 405 nm for visualization of Alexa 488, Alexa 568 and DAPI, respectively.
The microscopic images were quantitatively analyzed by ImageJ 1.52b (U.S. National Institutes of Health, Bethesda, MD, USA) to detect the difference in protein expression between different conditions. The intensity of the fluorescence in every photo was measured by ImageJ after the areas of interest were defined by the wand (tracing) tool. Furthermore, all the values were normalized to background fluorescence.

31st DLR Parabolic Flight Campaign
The parabolic flights were performed from the Bordeaux-Mérignac Airport between 6 and 9 March 2018. The cells were transferred on board of the Airbus 310 to a 37 • C pre-warmed incubator shortly before take-off and they were incubated at 37 • C for the whole time of the flight. The parabolic flight consisted of 31 parabolas. Each parabola had an initial phase of hyper gravity (1.8 g) for 22 s during pull up, followed by a microgravity phase for 22 s. At the end of the parabola, there is a second phase of hyper gravity for 22 s during pull out. The flight maneuver is repeated 31 times per flight day [11] (Figure 12).

RNA Isolation and qPCR
During the parabolic flights, the MCF-7 cells were fixed with RNAlater (Invitrogen by Thermo Fischer Scientific) at the end of the first parabola (P1) and the end of the last parabola (P31). The cells were cultured in T-75 cell culture flasks (75 cm 2 , SARSTEDT) with 10 mL medium in each flask. Each flask had a fixed three-way connector on the lid which was connected with 140 cm tubing to a 50 mL syringe filled with RNAlater. The RNAlater was injected manually into the flasks at the designated times. Additional MCF-7 cells were incubated on ground to serve as a ground control. The ground control cells were fixed with RNAlater in parallel to the samples on board of the flight. After landing, the medium and RNAlater mixture were thrown away and replaced with 3-5 mL of fresh RNAlater. Cells were harvested with 25 cm scraper (SARSTEDT) and incubated with RNAlater at 4 • C in 15 mL tubes until RNA isolation.
All the falcon tubes were centrifuged (2500 g for 10 min at 4 • C), followed by discarding the supernatant. The RNA was isolated afterwards by the RNeasy Mini Kit (Qiagen) according to the manufacturer's protocol. The quality of the RNA was evaluated with a spectrophotometer. The RNA was converted to cDNA with a High Capacity cDNA reverse Transcription Kit according to the manufacturer's protocol (Applied Biosystems, Darmstadt, Germany). The the final volume of the reverse transcription reaction mix was 20 µL with 1 µg total RNA added to each reaction mix. The primers were designed using Primer Blast (primer designing tool from NCBI).
A total volume of 13 µL SYBR green reaction mix (Applied Biosystems) was pipetted in each well in a 96 well plate. 1 µL of cDNA was added to each reaction mix with a concentration of 100 µM forward and reverse primers. 7500 Fast Real-Time PCR System (Applied Biosystems) was used to determine the transcription level of targeted genes ( Table 2). The program consisted of initial 20 s holding stage of 95 • C followed by cycling stage. The cycling stage consisted of 40 cycles of 3 s at 95 • C and 30 s at 60 • C. A melt curve stage was implemented at the end which consisted of 15 s at 95 • C and 60 s at 60 • C. The data were collected and analyzed by the ∆∆CT method; 18s and TBP were used as reference genes [21]. Table 2. List of all the primer sequences used in the quantitative PCR. All the sequences are listed from 5 -3 direction.

Western Blot Analysis
Western blot analysis, gel electrophoresis, trans-blotting, and densitometry were carried out following routine protocols as described previously [38][39][40]. Following lysis and centrifugation, aliquots of 30 µg were subjected to SDS-PAGE and Western blotting. The samples attained at the end of the P1 and P31 are compared to 1g control samples. Each condition is represented with 4 samples with a total number of 12 samples for all the conditions. The samples were loaded on Criterion XT 4-12% precast gels (Bio-Rad, Hercules, CA, USA) and run for 1h at 150 volts. Proteins were then transferred with a TurboBlot (Bio-Rad) (100 V, 30 min) to a PVDF membrane. Glyceraldehyde -3-phosphate-dehydrogenase (GAPDH) was used as a loading control. Membranes were then blocked for two hours in TBS-T containing 0.3% I Block (Applied Biosystems, Foster City, CA, USA). For detection of the selected antigens (see Table 3), the membranes were incubated overnight at room temperature in TBS-T and 0.3% I Block solutions of the antibodies. Following three washing steps of 5 min, membranes were incubated for additional two hours at room temperature with secondary antibody horseradish peroxidase (HRP)-linked antibody (Cell Signaling Technology Inc., Danvers, MA, USA) diluted 1:4000 in TBS-T and 0.3% I-Block. The respective protein bands were visualized using Bio-Rad Clarity Western ECL (Bio-Rad) and images were captured with Image Quant LAS 4000 mini (GE Healthcare Life Science, Freiburg, Germany). Images of stained membranes were captured on Syngene PXi 4EZ image analysis system (Synoptics, Cambridge, UK) and analyzed using the ImageJ software for densitometric quantification of the respective bands and total protein load [22]. Approximately 20,000 MCF-7 cells were seeded into Ibidi slide flasks two days prior to the flight day. Four flasks were fixed at the end of the first parabola and additional four flasks were fixed at the end of the 31st parabola. Four slide flasks were cultured in parallel on ground to act as a control. Cells were fixed with 4% PFA and transferred to the lab to continue the staining procedure. MMP9, IL 6 and IL-8 were used as primary Antibodies. Alexa Fluor plus 488 goat anti-mouse IgG was used as a secondary antibody. DAPI and phalloidin were used additionally in all the slides ( Table 1). The immunostaining procedure was performed as mentioned earlier [22].

Statistical Analysis
GraphPad prism 7.01 (GraphPad Software, Inc., California, USA) was used to analyze the data. The nonparametric Mann-Whitney U test was used as a statistical test of significance. The difference between groups was considered significant when the P-value was less than 0.05.

Conclusions
The FLUMIAS microscope has now been shown to be an elegant device suitable for live-cell imaging in real microgravity [11,30]. We could show for the first time, significant changes in the F-actin and microtubule cytoskeleton on living MCF-7 breast cancer cells in orbit. MCF-7 cells sense microgravity early and focal adhesion proteins are involved in this process. The actin cytoskeleton is contributing to adhesion and migration of the cancer cells. The early formation of lamellipodia and filopodia is the right step in this direction [66]. Early increases in VEGFA and CXCL8 gene expression as well as the down-regulation of VCL mRNA and the reduced E-cadherin protein indicate a change to a more invasive function of the MCF-7 cells exposed to short-term microgravity which supports earlier data with thyroid cancer cells exposed to parabolic flight maneuvers [16]. Our future plan is to investigate these cells for a longer time in space to investigate the behavior of breast cancer cells on the ISS.

Conflicts of Interest:
The authors declare no conflict of interest.