NT, 3-methyladenine (3MA), and VPS34 IN were supplied by MedChemExpress (NJ, United States). The NT sample was dissolved in normal saline (Xie et al., 2019). Primary antibodies to Beclin-1, VPS34, LC3B, P62, CD34, SOD1, eNOS, and HO-1 were bought from Abcam (Cambridge, United Kingdom). Primary antibodies to VE-cadherin and VEGF were supplied by Affinity Biosciences (OH, United States) and primary antibodies to LC3 I/II were bought from ZenBio (Chengdu, China). Anti-mouse and anti-rabbit secondary antibodies IgG-conjugated with Alexa Fluor 488 (green) and Alexa Fluor 594 (red), or with horseradish peroxidase (HRP), were obtained from Abcam (Cambridge, United Kingdom). Umbilical vein endothelial cells were bought from OTWO (Shenzhen, China). RPMI 1640 medium (1640) and fetal bovine serum (FBS) were bought from Gibco (California, United States).

Umbilical vein endothelial cells (UVECs) were cultured in RPMI 1640 complete medium containing 10% serum. The cells were divided into four groups: the control group, the H₂O₂ group (added 100 μM H₂O₂), the NT group (added 100 μM H₂O₂ + 100 μg/ml NT), and the NT + VPS34 IN group (added 100 μM H₂O₂ + 100 μg/ml NT + 10 nM VPS34 IN).

The UVECs were laid on a 12-well petri dish and cultured overnight until a fused monolayer was formed. The cells were scratched with a 200-μL pipette and washed with phosphate-buffered saline (PBS) three times. The images of monolayers of injured cells were captured using light microscopy at 0, 6, 12, and 24 h post-injury. UVECs were laid onto 96-well plates with 10,000 cells per well. After 12 h, the cells were divided into three groups: the control group, the 50 μg/ml NT group, and the 100 μg/ml NT group. The CCK-8 kit was used to detect cell proliferation.

Sixty healthy C57BL/6 male mice (20–22 g) were provided by the Experimental Animal Center of Wenzhou Medical University. The animal experiment was approved by the Animal Protection and Use Committee of Wenzhou Medical University (Wydw. 2021-0242). These mice were randomly divided into 4 groups, including the control group, NT-treated group (NT group), NT+3MA treated group (NT+3MA group), and NT + VPS34 IN–treated group (NT + VPS34 IN group). Prior to surgery, all mice were anesthetized by 1% sodium pentobarbital (50 mg/kg, i.p.). The random dorsal flap was constructed by removing all the blood-supplying arteries from the central back of the mouse with an aspect ratio of 8:3. Finally, the detached flap was fixed. The mice were killed on the seventh day after surgery. After euthanasia, the skin flap tissue and substantial organs were immediately collected for follow-up experiments.

The mice in the NT and NT+3 MA groups were treated with 40 mg/kg/d NT intraperitoneal injection for 7 days and the control group was treated with an unequal volume of saline. The mice in the NT+3MA group received 15 mg/kg/d 3MA 30 min before NT through intraperitoneal injection. The mice in the NT + VPS34 IN group received 5 mg/kg/d VPS34 IN 30 min before NT through intraperitoneal injection.

Three and seven days after surgery, the survival of the flap was observed using high-quality photography. The macroscopic development, appearance, and color characteristics of the flaps were observed 7 days after surgery. All images were measured using ImageJ (MD, United States). To calculate the survival area, the survival area percentage was measured as follows: survival area range/total area × 100%.

Seven days after surgery, the skin flaps were collected from each group and weighed. Then, they were dehydrated until the weight remained stable. The degree of edema can be determined as follows: ([wet weight − dry weight]/wet weight) × 100%.

LDBF imaging was used to determine the blood supply and vascular flow of the flap. Under anesthesia, the mouse lies in the prone position in the scanning area, and the laser Doppler imager scans the entire flap area. The blood flow at 0, 3, and 7 days was observed postoperatively through the color of the live blood flow images provided. The quantification of blood flow was performed via perfusion units, and the blood flow was measured using moorLDI Review software (version 6.1).

Tissue samples were taken from each group for pathologic analysis. The tissue was fixed with 4% paraformaldehyde and embedded in paraffin, cut into 5 μm for H and E and Masson’s trichrome staining. H and E–stained sections were examined under a light microscope (x 10) to assess histological changes, including granulation tissue, swelling, and microvascular remodeling. Masson-stained sections were examined under a light microscope (x 10) to assess fibrotic accumulation.

The primary antibodies against LC3B (1:500), P62 (1:1,000), CD34 (1:300), eNOS (1:200), and SOD1 (1:200) were used. Next, the tissues were washed with PBS three times. Then, the corresponding secondary antibodies (1:1,000) were applied for 1 h. The tablets were washed three times with PBST and were finally sealed with a sealing solution containing DPAI. A Nikon ECLIPSE Ti microscope (Nikon, Tokyo, Japan) was used to take images. Single dyeing uses grayscale display and double dyeing uses color display.

The extracted protein was determined by Coomassie bright blue method, and the protein sample was prepared with a concentration of 40 μg/20 μLl. After electrophoresis, the proteins were transferred onto polyvinylidene fluoride (PVDF) membranes (Bio-Rad, Hercules, CA, United States). The membrane was pre-incubated with 5% milk (Bio-Rad) for 2 h and incubated with each of the following antibodies: anti–Beclin-1 (1:500), anti-VPS34 (1:1,000), anti-LC3 I/II (1:1,000), anti-P62 (1:10,000), anti–HO-1 (1:1,000), anti-SOD1 (1:3,000), anti-eNOS (1:2000), anti-VEGF (1:500), anti–VE-cadherin (1:500), anti-CD34 (1:500), and GAPDH (1:3,000) at 4°C for 12 h. After that, the membranes were washed with TBST three times and incubated with secondary antibodies for 90 min. The signals were detected using ChemiDoc XRS + Imaging System (Bio-Rad).

The blood of mice was collected by anticoagulant vessels containing heparin lithium, and the supernatant plasma was collected after centrifugation at 3,000 r at 4°C for 5 min. 100 μL of plasma was poured into a blood biochemistry tray (Micro-nano Chip, Tianjin, China) and diluted with 430 μL of pure water. An M3 biochemical analyzer was used (Micro-nano Chip, Tianjin, China) to test related indexes on the test tray with better density.

Statistical analysis was performed using a two-sided Student’s t-test. SPSS13 was used for statistical analyses. Data were expressed as mean ± standard deviation (SD). p < 0.05 was considered statistically significant.

NT is the active extract of Panax notoginseng (Figure 1A), which can promote blood circulation, remove blood stasis, and increase blood flow. The proliferation, migration, and remodeling of vascular endothelial cells are crucial in random flap transplantation. We first tested the migration ability of UVECs by the cell scratch test, and the experimental results showed that the migration ability of UVECs was significantly decreased after H₂O₂ stimulation than the control group, and the migration ability of UVECs was well-recovered after NT treatment (Figures 1B–C). Then, we used the CCK-8 test to detect UVEC proliferation by NT, and the experimental results showed that NT could effectively promote the proliferation of UVECs (Figure 1D). Furthermore, we detected the toxicity of NT in vivo, and no obvious pathologic changes were found in the brain, kidneys, spleen, and other tissues by H and E staining (Figure 2A). The fluctuation of AST, ALT, and CRE in blood biochemistry was found to be within a normal range (Figure 2B). In conclusion, NT can promote cell proliferation and migration with minimum toxicity.

The distal end of the random flap is prone to ischemic necrosis because the pedicle of a blood vessel is cut off during modeling (Figure 3A). We first observed the necrosis of the flap and quantified the necrotic area. Our results showed that small areas of necrosis began to occur in the flaps of each group 3 days after surgery, and the survival of the flap in the control group was less than that in the NT and NT+3MA groups (Figures 3B–C). The flap survival rate in the NT group was higher than that in the NT+3MA group. On the seventh postoperative day, a large area of skin flap necrosis occurred in both the control and NT+3MA groups, while the survival rate of the NT group was better than that of the other two groups (Figures 3D–E). Our results suggest that NT can effectively promote the survival of random flaps, and the pro-survival effect may be related to autophagy activation.

Adequate blood perfusion is the key to flap survival, and LDBF was used to trace the microvascular network reconstruction. Our results showed that the random flaps in each group lost blood supply after modeling, and the blood flow signal in the NT and NT+3MA groups rebounded on the third day after surgery, as well as the blood flow signal in the NT group was higher than that in the NT+3MA group (Figures 4A–D). On postoperative day 7, blood flow signals in the NT group showed significant recovery among the three groups. The control and NT+3MA groups showed no significant recovery compared to the third postoperative day (Figures 4E,F). In conclusion, NT can effectively restore random flap perfusion and promote flap survival.

Neovascularization is the key to increase blood perfusion. We used histologic staining to observe the blood supply regeneration of random flaps. H and E staining showed no obvious neovascularization in the flap of the control group. On postoperative day 7, the NT group showed a large number of microvessels. The number of microvessels in the NT+3MA group was less than those of the NT group (Figures 5A,B). Masson’s trichrome staining showed that the NT group had angiogenesis and collagen fiber arrangement was dense and in order, while the collagen fiber arrangement was irregular and loose in the control and NT+3MA groups (Figure 5C). Then, we assessed the degree of edema in the flap, and the results showed that the degree of edema in the NT group was lower than that in the control and NT+3MA groups (Figure 5D). In conclusion, NT could effectively improve the blood perfusion and tissue morphology of random flaps to promote the survival of flaps.

Western blotting was used to further analyze the expression of neovascularization. Our results showed that the CD34 index representing neovascularization significantly increased after NT treatment, and the number of neovascularization in the NT+3MA group was significantly reduced than that in the NT group (Figures 6A,B). The expression levels of VEGF promoting angiogenesis and VE-cadherin promoting vascular maturation were also significantly increased in the NT group compared with those of the control group. The levels of VEGF and VE-cadherin in the NT+3MA group were significantly lower than those in the NT group (Figures 6A,C,D). Then, the oxidative stress levels of random flaps were analyzed by Western blotting. We detected eNOS, HO-1, SOD1, and other reductive indexes and found that the expression of reductive indexes in the NT+3MA group was significantly higher than that in the control group after NT treatment, and the expression of reductive indexes in the NT+3MA group was significantly lower than that in the NT group (Figures 6E–H). In summary, NT can effectively promote angiogenesis, maintain the stability of regenerated blood vessels, and promote vascular recanalization to form an arteriovenous loop. Moreover, it can promote the generation of reducing substances to reduce the damage caused by oxidative stress.

In random flaps, autophagy is needed to generate energy to supply cell survival due to the lack of vascular pedicle and tissue blood supply. Therefore, the activation of autophagy can effectively promote the survival of flaps. We first detected autophagy-related proteins, namely, Beclin-1, VPS34, LC3, and P62 using Western blotting. We found that the autophagy activation indexes, namely, Beclin-1, VPS34, and LC3 in the NT group were significantly higher than those in the control group. Beclin-1 in the NT+3 MA group was significantly higher than that in the control group after autophagy inhibitor 3MA. The expression levels of VPS34 and LC3 were significantly downregulated (Figures 7A–D). P62 as a substrate for autophagy decreased significantly in the NT group than in the control group. The level of P62 in the NT+3MA group was significantly higher than that in the NT group (Figures 7A,E). Then, we further verified the expression of LC3B and P62 in each group by immunofluorescence. Our results showed that LC3B in the NT group was significantly higher than that in the control group, and the LC3B level in the NT+3MA group was significantly lower than that in the NT group. The results of P62 are exactly the opposite of those of LC3B (Figures 7F–H). In summary, NT promotes the survival of random flaps through the Beclin-1/VPS34/LC3 pathway.

To verify the autophagy pathway of NT action, the VPS34 inhibitor: VPS34 IN was first used to inhibit the expression of VPS34 at the cellular level. Western blotting results showed that the expression of VPS34 activated by NT was downregulated after VPS34 IN, LC3 expression was also downregulated, and P62 expression was increased. The expression levels of CD34, an indicator of angiogenesis, and eNOS and SOD1, an indicator of oxidative stress protection, were down-regulated after using VPS34 IN (Figures 8A–F). CCK-8 results showed that VSP34 IN significantly inhibited the protective effect of NT on UVECs (Figure 8G). Next, we used immunofluorescence to detect the expression of autophagy, angiogenesis, and oxidative stress protectants in tissues. Our results showed that VPS34 IN inhibited autophagy, reduced angiogenesis, and downregulated the expression of oxidative stress–protective substances (Figures 9A–I). The cell scratch assay showed that VPS34 IN could significantly inhibit the migration activity of UVECs (Figures 9J,K). In conclusion, NT activates autophagy in random flaps through the Beclin-1/VPS34/LC3 pathway, promoting the survival of flaps.