Electron Transfer Flavoprotein (ETF) α Controls Blood Vessel Development by Regulating Endothelial Mitochondrial Bioenergetics and Oxygen Consumption

While impairment of vascular homeostasis induced by hypercholesterolemia is the first step of cardiovascular diseases, the molecular mechanism behind such impairment is not well known. Here, we reported that high-cholesterol diet (HCD) induced defective vessel sprouting in zebrafish larvae. Electron transfer flavoprotein subunit α (ETFα) (encoded by the ETFA gene), a protein that mediates transfer of electrons from a series of mitochondrial flavoenzymes to the respiratory chain, was downregulated in HCD-fed zebrafish and in endothelial cells treated with oxidized low-density lipoprotein. Knockdown of ETFα with morpholino antisense oligonucleotides reproduced vascular sprouting defects in zebrafish larvae, while replenishing with exogeneous ETFA mRNA could successfully rescue these defects. ETFA knockdown in endothelial cells reduces cell migration, proliferation, and tube formation in vitro. Finally, knockdown of ETFA in endothelial cells also reduced fatty acid oxidation, oxygen consumption rate, and hypoxia-inducible factor-1α (HIF1α) protein levels. Taken together, we demonstrate that downregulation of ETFα is involved in hypercholesterolemia-induced defective vessel sprouting in zebrafish larvae via inhibition of endothelial proliferation and migration. The molecular mechanism behind this phenomenon is the decrease of HIF1α induced by downregulation of ETFα in endothelial cells. This work suggests that disturbance of ETFα-mediated oxygen homeostasis is one of the mechanisms behind hypercholesterolemia-induced vascular dysfunction.


Introduction
Hypercholesterolemia has been linked to cardiovascular disease (CVD) for decades, which could lead to premature atherosclerosis-based cardiovascular diseases and death, but the underlying mechanism is still far away from elucida-tion [1,2]. In our previous work, we utilized high-cholesterol diet-(HCD-) fed zebrafish larvae to mimic hypercholesterolemia and preatherosclerosis to investigate the molecular mechanism between hypercholesterolemia and atherosclerosis [3,4]. The zebrafish larvae fed a HCD acquired a broad spectrum of phenotypes which include not only hypercholesterolemia and atherosclerotic plaques like lesions but also delayed development and vascular deformities at 15 days postfertilization (dpf). Importantly, the severity of deformities like vascular defects was positively correlated with the increase of cholesterol concentration in diet, which suggests that hypercholesterolemia compromises the vessel development. Endothelial cells play an important role in the formation of vessel under both physiological and pathological conditions [5]. As damage of the endothelium is considered as the initiation step of atherosclerosis, it is necessary to investigate the relationship between hypercholesterolemia and vascular deformities in zebrafish. iTRAQ analysis of normal-and HCD-fed zebrafish larvae found a total of 63 differentially expressed proteins [3]. More than 12.2% of those 63 candidates were metabolic activities related, and 14.3% of them were mitochondrion located, which suggest that mitochondria are probably related to hypercholesterolemia and deformities. However, the differentially expressed mitochondrion elements is a driving force of those phenotypes or just a subsequent bystander adaptation needs further investigation. Although the volume of mitochondria in endothelial cells is not abundant as some cell types like hepatocytes, the importance of mitochondria in EC homeostasis is receiving more and more attention [6][7][8][9]. Recently, there are many studies that revealed that endothelial metabolism is a key driver of vessel sprouting in addition to well-known growth factor-based signaling [8,9]. Endothelial mitochondria are found not only as a supplier of energy but also as a signal station getting involved in many biological activities like angiogenesis [10,11]. To reveal the relationship between mitochondrion function and hypercholesterolemia-related vascular deformities, we pick electron transfer flavoprotein-α (ETFα), one of the differentially expressed mitochondrial proteins in iTRAQ analysis, to carry out our investigation. ETFα is an α subunit of dimeric enzyme which locates in the mitochondrial matrix space and collects reducing power from multiple metabolic pathways, funneling electrons into the respiratory chain [12]. Its central position in mitochondrial bioenergetics enables ETFα an appropriate candidate to evaluate the role of mitochondria in vascular development and homeostasis. Loss of function in ETF could induce severe symptoms, the so-called multiple acyl-CoA dehydrogenase deficiency (MADD), in human beings [12][13][14][15]. Many patients with ETF deficiency are neonatal lethal and only a fraction of patients with milder signs survives to adulthood [12][13][14][15]. The severity of the symptoms induced by ETF deficiencies depends on the residual enzyme activity [12,16]. To mimic the milder downregulation of ETFα induced by hypercholesterolemia but not severely demolished like MADD, we use morpholino to knockdown ETFA in zebrafish embryos to leave residual ETFA function. Injection of ETFA morpholino led to less than 42% mortality at 48 hpf in zebrafish larvae, and the surviving larvae had a broad spectrum of deformities, which include vascular malformation. Knockdown of ETFα in endothelial cells with shRNA could reduce cell migration, proliferation, and tube formation in vitro. The fatty acid oxidation (FAO), oxygen consumption rate, and HIF1α protein expression were also impaired by ETFA knockdown. Our work provides first-hand evidence to support a critical role for ETFα or mitochondria in vessel sprouting and development. This work may shed light on the underlying link between hypercholesterolemia and CVD.

Materials and Methods
2.1. Culture and Maintenance of Zebrafish Larvae. The adult zebrafish (Danio rerio) were maintained with an automatic fish housing system at 28°C following standard protocols. Transgenic lines Tg (Flk: eGFP) were obtained from Professor Yiyue Zhang at South China University of Technology. Zebrafish embryos and larvae were raised in 10% egg water under a 14 h-10 h light-dark cycle, and 0.003% 1-phenyl-2thiourea (PTU) (Sigma, P7629) was added to the egg water since 24 hpf to prevent pigment formation.
2.2. iTRAQ Data Analysis. The procedure of isobaric tags for relative and absolute quantitation (iTRAQ) is described previously. The MS/MS raw data were blasted against the Ensembl Danio Rerio database for peptide identification and quantification using Mascot 2.3.02. Proteins with FDR ≤ 0:01 were qualified for further quantification. A fold change cutoff ratio (FC) of ≥1.2 or ≤0.833 was set as the threshold to identify differently expressed proteins. To calculate the fold change between sample A and sample B, the formula is as follows: FC, k = RAk/RBk (R denotes the relative quantitative value of the protein, k denotes the protein, A and B denote different groups, and RAk and RBk denote the relative quantitative values of protein k in groups A and B. Student's t-test was performed with the relative quantitative value of the peptide on each protein to judge the significance of differentially expressed proteins between groups, and the default P value was <0.05. To make the data obey the normal distribution, the relative quantitative value of peptides needs log2 transformation. The calculation formula is as follows: Pk = t:testðlog2ðUAjÞ, log2ðUBjÞ, j ∈ kÞ (U denotes the relative quantitative value of the peptide; j denotes the peptide). The differentially expressed proteins were annotated with Gene Ontology (GO) annotation. QPCR and Western blot were carried out to confirm the data from iTRAQ analysis.

Morpholino and mRNA Injection. Morpholinos (MOs)
were purchased from GeneTools (Philomath, OR, USA) and dissolved in DEPC water. Morpholinos were designed to prevent ETFA splicing (ETFA MO) by targeting the exon 3-intron 2 junction. Zebrafish embryos were microinjected with 5 ng ETFA or control MO at a one-cell stage. The respective MO sequences are ETFA MO: 5′-GCTCTGCAA CCTGTGCAAAATGAGA-3′; control MO: 5′-CCTCTT ACCTCAGTTACAATTTATA-3 ′ . The overexpression ETFA-mRNA was obtained from the in vitro transcription of ABSR-RNA by using the mMESSAGE mMACHINE™ SP6 Transcription Kit (Invitrogen™, AM1340). PCS2+ vector (Addgene, MA, USA) was used to construct a plasmid with the ETFA-CDS sequence, and ETFA-mRNA was obtained by HpaI digestion, followed by in vitro transcription. We injected 50 pg, 100 pg, 200 pg, and 500 pg mRNA or/and 5 ng MO at the one-cell embryo stage. 2.5. In Vivo Confocal Microscopy. For in vivo confocal microscopy, zebrafish larvae were anesthetized with 0.02% tricaine and mounted in 0.5% low-melting agarose and observed with an Olympus FV1000 confocal laser scanning microscope (Olympus, Tokyo, Japan). Images of zebrafish larvae were captured every 200 nm and analyzed using the Olympus FluoView software. The Z-step of imaging was 10 μm. Quantitative analysis of the ISVs and its morphology was conducted following the processes described in reference [17].
2.7. Lentivirus Transfection. HUVECs were seeded in 6-well plates overnight with a density of 1 × 10^5 and infected with control or gene-specific lentivirus (MOI: 10). At 18-24 h postinfection, the infection medium was replaced with DMEM containing 10% FBS and cells were cultured for further 24-48 hours.
2.8. Tube Formation Assay. Matrigel (BD Bioscience) (150 μl) was added to the 48-well plate precooled at 4°C and incubated at 37°C for 2 h in a 5% CO 2 incubator. Cells were dissociated into single cells and added onto the solidified Matrigel at a density of 2:5 × 10^4, followed by an incubation at 37°C for 3-6 h. The tube formation was observed by a microscope. Networks of tube-like structures were measured using ImageJ software.
2.9. Wound Healing Assay. After planting the virus-treated cells in 6-well plates and growing to 95% confluence, a neat line was drawn in each well using a sterile 200 μl pipette tip. Cells were washed twice with PBS and immediately photographed as "S0" after adding fresh culture medium in the absence or presence of 2 μM mitomycin C (2 μM). Sixtwelve hours later, cells were photographed again and used as "Sx." NIH ImageJ software was used to measure the wound healing area (the gap area at S0 minus the gap area at Sx).

Fatty Acid Oxidation Assay.
Oxidation of exogenous and endogenous fatty acids was measured using the XF Palmitate-BSA FAO Substrate with the XF Cell Mito Stress Test. Cells were seeded at 40,000 cells per well on Seahorse XF96 cell culture plates (Seahorse Bioscience Europe, Copenhagen, Denmark). The measurement of oxygen consumption was performed at 10 min intervals (2 min mixing, 2 min recovery, and 6 min measuring) for 3 h using the Seahorse XF96 analyzer.
2.11. Protein Extraction. 1 to 3 dpf zebrafish embryos were collected by breaking their membranes and adding 0.3 mM PMSF to remove yolk sac, followed by centrifugation at 200 × g at 4°C for 5 min. The treated embryos or cells were washed with PBS, and proteins were extracted by using RIPA lysis buffer (Beyotime, China), with protease and phosphatase inhibitors. Following centrifugation of the lysates at 13,000 × g at 4°C for 10 min, the supernatants were collected and protein concentrations were quantified using a BCA assay kit (Beyotime, China).

Western
Blot. Equal amounts of protein from each sample were separated by 10% SDS-PAGE and transferred to PVDF membrane which were blocked with 5% skimmed milk (Sigma-Aldrich; Merck KGaA) in TBS solution with 0.1% Tween-20 (Sangon Biotech Co. Ltd.) at room temperature for 1 h and then incubated with the primary antibodies (1 : 1000) at 4°C overnight with rocking. The membrane was washed with TBST for 5 min 3 times and incubated with the secondary antibody (1 : 5000) at room temperature for 1 h. The reactive bands were detected and observed via an enhanced chemiluminescence (ECL) kit. Densitometric quantifications of bands were done with ImageJ software (National Institutes of Health) using GAPDH or β-actin as an internal reference.

High-Cholesterol Diet Impairs Vessel Development in
Zebrafish Larvae. Feeding a high-cholesterol diet (HCD) to Tg Flk1: eGFP zebrafish larvae for 10 days was used to mimic atherosclerosis-like phenotypes in vivo, as previously reported [3]. Expectedly, it was found that HCD contained different concentrations of cholesterol which caused a trend of developmental delay, which is characterized with decreased body length and with significant shorter body length in zebrafish larvae fed a 10% cholesterol diet (Figures 1(a) and 1(b)). Importantly, we observed that both the number and length of the blood vessels in caudal fins were significantly decreased by HCD feeding in a dosedependent manner (Figures 1(c)-1(e)). And the angiogenesis-related gene HIF1 was also decreased in HCD-fed larvae (Figure 1(g)).
3 Oxidative Medicine and Cellular Longevity  Oxidative Medicine and Cellular Longevity

High-Cholesterol Diet Reduces the ETFα Protein Level in
Zebrafish. In order to reveal the differences of protein profiles between normal and atherosclerotic zebrafish larvae (diet fed containing 4% cholesterol), the tissues of the two groups mentioned above were subjected to iTRAQ analysis, as described in our previous study [3]. After reanalyzing of the iTRAQ data, it was found that several mitochondrionrelated proteins were differentially expressed (Table 1). ETFα is one of those mitochondrion-related proteins. Data from RT-qPCR (Figure 1(f) and Figure S2) revealed that ETFα is the only one that downregulated in 4% to 10% HCD-fed zebrafish larvae and consistent with the result

Knockdown of ETFα Caused Vessel Developmental
Defects in Zebrafish Larvae and Such Defects Were Rescued by Exogenous Zebrafish ETFA mRNA. An ETFA-specific morpholino oligonucleotide was designed to knockdown ETFα expression in zebrafish larvae. This ETFA-specific morpholino specifically binds to its complementary 25-base target RNA sequence at the junction site between intron 2 and exon 3 in the zebrafish ETFA pre-mRNA and interferes in mRNA splicing ( Figure S1A). PCR data showed that injection of 5 ng ETFA-MO could significantly reduce ETFA gene expression at both 24 and 48 hours postfertilization (hpf) ( Figure S1B). As expected, a much higher mortality was observed in ETFA-MO-injected embryos (Figure 2(a)). Importantly, it was found that ETFA knockdown in live embryos caused a broad spectrum of malformations including delayed development of embryos, defective vessel sprouting, short body, spinal curvature, and curly tail at different time points (Figures 2(b) and 2(c)). Quantitative analysis of these defects showed that ETFA MO-injected embryos exhibited a significant high percentage of defective vessel development (80%) (Figure 2(d)). The defects of vessel development were classified with different severities: incomplete DLAVs (slight), short ISVs (moderate), and inadequate sprouting (severe) at 32 hpf (Figures 3(a) and  3(b)). Accordingly, we found that the number of intact ISVs in the ETFA-MO group was much less than those of the

OxLDL Reduces the Protein Level of ETFα in Endothelial
Cells. 7-Keto cholesterol (7-keto) is a bioactive sterol and a major oxysterol component of oxidized low-density lipoprotein (oxLDL). It was found that 7-keto could reduce the protein level of ETFα in HUVECs in a dose-dependent manner ( Figure 6(a)). Proteasome inhibitor MG-132 had no effect upon decrease of ETFα protein expression levels induced by 7-keto treatment, suggesting that the regulation of ETFα protein expression by 7-keto is independent of the proteasome pathway. As expected, both 7-keto and ETFA shRNA lentivirus could inhibit EC tube formation significantly with reduced total tube length (sum of branches and segment length per image) and junctions (number of junction per image) (Figures 6(c) and 6(d) and Figure S2B). This result suggests that downregulation of ETFα is related to the EC damage induced by oxLDL.

Knockdown of ETFα Inhibits Endothelial Migration and
Proliferation. The coordination of EC migration and proliferation is essential for both physiological angiogenesis and pathological angiogenesis. Hence, scratch wound assay was utilized to evaluate the importance of ETFα in cell proliferation and migration. It was found that knockdown of ETFα significantly inhibited wound closure in endothelial cells at 20 hours postscratching when mitomycin C, a cell proliferation inhibitor, was absent ( Figure 6(e) and S2). However, the wound healing abilities of control, scramble shRNA-treated, and ETFA knockdown ECs were not significantly different      when mitomycin C was present, which suggests that the effect of ETFα knockdown on wound healing is less pronounced when cell proliferation is inhibited. To elucidate whether endothelial migration and proliferation are influenced by ETFA knockdown, we carried out transwell migration assay and Edu proliferation assay; the results showed that knockdown of ETFα reduces both cell migration and proliferation significantly (Figures 6(f) and 6(g) and Figure S2C, D) but the proliferation was influenced more dramatically.

Knockdown of ETFα Reduces the Fatty Acid Oxidation and Oxygen Consumption in HUVECs.
It is reported that ECs utilize carbons produced by FAO to fuel biomacromolecule synthesis, which is vital and necessary for cell proliferation [18]. With the combination of XF Palmitate-BSA (Palm-BSA) (FAO substrate), etomoxir (Eto) (an irreversible inhibitor of FAO), and the Seahorse XF Cell Mito Stress Test, the relative utilization of exogenous and endogenous FAs in ECs was determined. In Figure 7(a), Eto plus BSA (green line) and BSA only (red line) were used to evaluate utilization of endogenous FA. Basal respiration (OCR) had no decline in the BSA + Eto group (green) compared with BSA only group (red). This indicates that under quiescent condition, the basal respiration of ECs was due to oxidation of other substrates rather than endogenous FAs. The Palm-BSA + Eto group (blue) was used to determine the oxidation of exogenous FAs. FCCP, a potent uncoupler of oxidative phosphorylation in mitochondria that disrupts ATP synthesis by transporting protons across cell membranes, was used for detecting maximal respiration in ECs. Data shown in Figure 7(a) revealed that compared with control-BAS (red line), a significant increase in maximal respiration was observed in the Palm-BSA group (purple line), while a significant decrease of maxi-mal respiration was observed in Eto + Palm-BSA (blue line) and Eto + BSA (green line) groups. This indicates that exogenous FA (as opposed to endogenous FA) is primarily being oxidized when a bioenergetic stress is applied into ECs. It also suggests that FAs are utilized as a primary energy source under stress. ETFα is required for normal mitochondrial FAO and normal amino acid metabolism in the liver [16]; however, its function in EC FAO is still not fully elucidated. We found that knockdown of ETFα in ECs significantly reduced the oxygen consumption rates (pmol O 2 /min/well) at baseline from 8-20 pmol O 2 /min/well in control ECs to 4-9 pmol O 2 /min/well in ETFA knockdown ECs (Figures 7(b) and 7(c)). Importantly, no significant increase was observed in terms of maximal respiration after ETFA knockdown (Figures 7(b) and 7(d)). This result suggests that the endothelial cells could not utilize fatty acid under bioenergetic stress when ETFα was knockdown, which indicates that ETFα plays an important role in FAO of endothelial cells. Additionally, the OCR was lower in ETFα knockdown cells than Eto-treated cells, suggesting that ETFα is participated in not only oxygen consumption of FAO but also other substrates. These data have collectively suggested that ETFα is important for EC FAO and mitochondrial respiration in ECs. The stability of HIF-1α was impaired when ETFα was knockdown in endothelial cells.
Hypoxia and the HIF-1α pathway are important regulators for EC angiogenesis. HIF-1α is stable under hypoxia but degraded under well-oxygenated condition; however, specific metabolic imbalances, or exponentially growing ECs, can accumulate HIF-1α in cells, even under normoxic conditions [19]. We have shown that knockdown of ETFα could reduce the oxygen consumption rate and EC tube formation, which prompted us to wonder if HIF-1α protein expression could be influenced by ETFA knockdown in ECs. Indeed, it was  HUVECs measured by the Seahorse XF analyzer, in which the oxygen consumption rate (OCR) over time is determined. BSA was used to assess utilization of endogenous fatty acid; Palm-BSA was used to assess utilization of exogenous fatty acid. Etomoxir is an inhibitor of fatty acid oxidation (FAO). Oligomycin, an ATP synthase (complex V) inhibitor, was added to detect cellular ATP production; FCCP, a potent uncoupler of oxidative phosphorylation in mitochondria, was added to assess maximal respiration of HUVECS; a mixture of rotenone, a complex I inhibitor, and antimycin A, a complex III inhibitor, was included to measure nonmitochondrial respiration in cells. (b) OCR profiles in ETFα knockdown HUVCEs; (c) basal respiration of control and ETFα knockdown HUVECs. OCRs in different groups were analyzed with one-way ANNOVA, * * * * P < 0:00001, n = 10; (d) maximal respiration of control and ETFA knockdown HUVECs. OCRs in different groups were analyzed with one-way ANNOVA, * * * P < 0:0001, * * * * P < 0:00001, n = 10; (e) representative immunoblot for HIF1α and ETFα in control-, scramble shRNA-, and ETFA shRNA lentivirus treated HUVECs. Cell lysates were collected at 24 hours or 48 hours after lentivirus transfection. Acetate was added to ETFα knockdown HUVECs. β-Actin was the loading control; (f) representative immunoblot for HIF1α and ETFα in control-, scramble shRNA-, and ETFA shRNA lentivirus-treated HUVECs. HUVECs were exposed to hypoxic condition for 12 hours before collection. Cell lysates were collected at 24 hours or 48 hours after lentivirus transfection.
found that HIF-1α protein expression was increased in control HUVECs under normal culture condition 48 hours after seeding (Figure 7(e)). However, ETFα knockdown significantly reduced HIF-1α protein expression. Acetate, which could compensate the lack of acetyl-CoA induced by FAO block in cells, could not increase the HIF-1α protein expression when ETFA was knockdown (Figure 7(e)). This result suggests that only compensating the product of FAO could not reverse the degradation of HIF-1α, which is mainly regulated by the O 2 level. It also indicates that defective vessel growth induced by ETFα knockdown not only is due to FAO block but also O 2 consumption related. We also observed that ETFα knockdown significantly reduced HIF-1α protein expression even under hypoxic condition (Figure 7(f)).

Discussion
The metabolic switch of endothelial cells is now considered an important driving force of physiological and pathological vascular events [6]. Mitochondria are in the central position of endothelial metabolic homeostasis through supplying energy, signaling, and material needed for biosynthesis [11]. Although mitochondria are not a major ATP source of angiogenic ECs, it still mediates oxidative phosphorylation (OXPHOS) via the electron transport chain (ETC) to produce ATP [5]. The leakage of electrons during ETC is also the major source of cellular ROS, which makes mitochondrion dysfunction important for vascular disease-like atherosclerosis [5,20]. Our work found that persistent hypercholesterolemia in zebrafish larvae could induce downregulation of several mitochondrion-and metabolic-related enzymes, ETF α is one of them, and knockdown of it resulted to defective vessel growth in vivo and vitro. Human ETF are α/β-heterodimeric FAD-containing proteins in the mitochondrion matrix space [12,16]. ETF functions as a hub taking up electrons from at least 14 flavoenzymes, feeding them into the respiratory chain [16]. Genetic mutations in the ETFA or ETFB genes cause the Mendelian disorder MADD, which comprises a series of severe symptoms due to energy depletion, impairment of glucose homeostasis and ketogenesis, and the toxic effects of substrates and metabolites [12]. Patient ETF deficiency in human beings is neonatal lethal, and only a fraction of patients with milder signs survives to adulthood [12,16]. Studies revealed the severity of the symptoms induced by ETF and ETF: QO enzyme deficiencies depend on the residual enzyme activity [12,16]. It is also proved by our unpublished work that complete deletion of ETFA is neonatal lethal to mice but knockdown of ETFA with morpholino could lead to less than 42% mortality at 48 hpf in zebrafish due to residual ETFA function. However, the surviving larvae had a broad spectrum of deformities, which include vascular malformation. These results suggest an important role of ETFα-related mitochondrial function not only in metabolism but also in the vascular homeostasis. ETFA and ETFB are persistently and highly expressed in most tissues, especially in the liver, heart, kidney, skeletal muscle, and fat tissue [12]. Although the ETFA and ETFB are very important for metabolic homeostasis, there is little literature about regulating the mechanism of the two genes' expression. Peroxisome proliferator-activated receptors (PPARs) are a highly potential regulator of ETFA and ETFB according to the bioinformatic prediction, and the former one is also an important regulator of fatty acid oxidation enzymes [12]. Our group will also focus on the relationship between PPARs and ETFA during angiogenesis next. Given the stable expression of ETF, its activity might be regulated by posttranslational modifications (PTMs). Our preliminary proteomics data and others' publication showed both that ETF-α and ETF-β subunits possess abundant PTMs, which comprises carbonylation, acetylation, glutarylation or succinylation, phosphorylation, and trimethylation [12]. However, the exact meaning and function of these PTM for ETF's activity are not clear and need further investigation.
The vascular system is a highly branched network that supplies surrounding tissues with oxygen (O 2 ) and nutrients [12,15,16]. Formation of the vascular network occurs from embryogenesis to adulthood and is stimulated by the oxygen and metabolism demands of organ growth and function [9]. The hypoxic tissues produce proangiogenic stimuli and initiate migration and proliferation of ECs in preexisting vessels to establish new vessels [16][17][18][19][20]. During this process, the migrating ECs utilize glycolysis to produce ATP and the proliferating ECs use FAO to supply the carbons needed for dNTP synthesis [10,24,25]. Once nutrient and O 2 supplies meet tissue demands, the sprouting process is terminated and ECs become quiescent [25]. ECs sense O 2 tension with many sensors, which include NADPH oxidases, endothelial nitric oxide synthase (eNOS), heme oxygenases, mitochondria, and 2-oxoglutarate-dependent iron(ii) dioxygenase superfamily [25]. These sensors interface with the hypoxiainducible transcription factor (HIF) family, which includes three isoforms HIFα (HIF-1-3) [26]. All three isoforms of HIFα can heterodimerize with the HIFβ/ARNT subunit to form an active transcriptional complex that initiates expression of hundreds of angiogenic genes [25]. The activity of these HIFs is regulated by the O 2 sensors, including prolyl hydroxylase domain proteins (PHD1-3) and factor inhibiting HIFs (FIH), all of which belong to the 2-oxoglutaratedependent iron (ii) dioxygenase superfamily [27]. During normoxia, PHDs use O 2 to hydroxylate specific proline residues of HIF proteins, which lead to degradation through the von Hippel-Lindau (VHL) E3 ubiquitin ligase complex-regulated proteasomal pathway [27]. Under hypoxia, HIFs become stable due to the reduction of PHD/FIH activity, triggering HIF's target gene expression, which subsequently regulate cell metabolism, proliferation, and angiogenesis [26,27]. However, there are exceptions. Such specific metabolic imbalances, or the cell culture density, can induce HIF1α accumulation, even under normoxic conditions through a not wellunderstood mechanism [19,28]. It is confirmed by our work that ETFα takes part in FAO; knockdown of which would influence endothelial proliferation more than migration. It is consistent with the statement that endothelial cell relies on glycolysis to supply energy when migrating, while needing FAO to provide materials for biosynthesis. Knockdown of ETFα would also reduce the protein level of endothelial HIF1α, which is in consistency with impaired vessel sprouting in ETFA MO-injected zebrafish larvae. The underlying mechanism behind it is probably related to O 2 consumption decrease in ETFA knockdown endothelial cells.