Naomaitai Ameliorated Brain Damage in Rats with Vascular Dementia by PI3K/PDK1/AKT Signaling Pathway

Background/Aims Naomaitai can improve blood perfusion and ameliorate the damage in the paraventricular white matter. This study was focused on observing the neuroprotective effect of Naomaitai on the vascular dementia of rat and exploring the action mechanism of PI3K/PDK1/AKT signaling pathway. Methods A vascular dementia model of rats was established by permanent, bilateral common carotid artery occlusion. Rats' behavior was tested by Neurological deficit score and the Morris water maze. The pathology and apoptosis were detected through HE staining and TUNEL assay. Myelin sheath loss and nerve fiber damage were detected by LFB staining. Inflammatory factors, oxidative stress, and brain damage markers were detected through ELISA. The expression of apoptosis-related proteins and PI3K/PDK1/AKT signaling pathway related proteins were measured by western blot. The expressions of PI3K, PDK1, AKT, and MBP in paraventricular white matter cells were detected by immunofluorescence. Results Naomaitai treatment decreased neurological function score in rats with vascular dementia, ameliorated paraventricular white matter damage caused by long-term hypoxia, and hypoperfusion reduced the brain injury markers S-100β and NSE contents, suppressed inflammatory reaction and oxidative stress, reduced IL-1β, IL-6, TNF-α, and MDA contents, and remarkably increased IL-10 and SOD contents. TUNEL and western blot assay showed that Naomaitai treatment decreased neuronal cell apoptosis, increased Bcl-2 expression, and reduced caspase-3 and Bax expression. Furthermore, we found Naomaitai inhibited PI3K and PDK1 expression and activated phosphorylated AKT protein in rats with vascular dementia. However, the protective effect of Naomatai in rats with vascular dementia was inhibited, and expression of PI3K signaling pathway-related proteins was blocked after administration of PI3K inhibitor. Conclusion Naomaitai can ameliorate brain damage in rats with vascular dementia, inhibit neuronal apoptosis, and have anti-inflammatory and antioxidative stress effects, which may be regulated by the PI3K/PDK1/AKT signaling pathway.


Introduction
Vascular dementia (VD) is a severe cognitive impairment syndrome caused by long-term hypoxia and hypoperfusion in the brain [1]. Cerebrovascular diseases, such as ischemic stroke, hemorrhagic stroke, and cerebral ischemia and hypoxia, are the main clinical causes for VD [2]. The aging of the social population makes VD a recognized public health issue [3]. VD is the second largest type of dementia after Alzheimer's disease. The research showed that longterm hypoxia and hypoperfusion in the brain region caused by the damage to the paraventricular white matter is the main factor of VD [4]. Therefore, white matter injury is also a unique clinical diagnostic basis for VD. The damaged areas showed pathological changes such as glial cell activation and proliferation [5]. Glial cell activation produced reactive oxygen species, which promoted the occurrence of oxidative stress [6]. In addition, cytokine secretion also stimulated inflammatory reaction and aggravated white matter damage [7]. Naomaitai (NMT) is a new type of traditional Chinese medicine developed by Guilin Sanjin Pharmaceutical Co., Ltd. NMT is composed of Sanchi, ginkgo leaf, Safflower and Danshen Root, etc. NMT can benefit vital energy, promote blood flow, stop endogenous wind, and reduce phlegm [8].
In the clinic, NMT is commonly used in the recovery period of ischemic stroke (cerebral infarction) [9][10][11]. Chinese medicine syndrome belongs to the meridian qi deficiency and blood stasis and wind phlegm and blood stasis to obstruct the arteries and veins. It has been proved that cerebral ischemia and hypoxia are the main cause of VD [5]. NMT can repair hypoxia and hypoperfusion and cognitive impairment in the rats' model of VD. NMT can play a protective role in the white matter of VD rats by improving the blood circulation of the brain [8]. And several studies have shown that most of the components of NMT have an effect on cerebral ischemia and hypoxia [12][13][14][15][16][17][18][19]. But no literature has reported the specific mechanism of the protective effect of NMT. This study explored the protective effect and mechanism of NMT on neurons and white matter in VD rat models, which may be associated with the PI3K/PDK1/AKT signaling pathway.

Model Preparation.
The rats were fasted but allowed free access to water 12 hours before surgery. The rats were anesthetized with 2% sodium pentobarbital 0.3 ml/100 g until rat's limbs were soft and the conjunctival reflex disappeared. The rats were fixed on the board in the supine position. After shaving on the neck and sterilizing with alcohol cotton, a median incision (approximately 1 cm) was made to bluntly dissociate fascia and subcutaneous tissue. The common carotid artery is located below the sternocleidomastoid muscle. The bilateral common carotid artery and vagus nerve were gently separated using a glass minute hand soaked in PBS buffer. The common carotid artery was permanently ligated at the distal end with a No. 4 surgical line. After the surgery, two drops of penicillin were dropped into the wound to prevent infection. The skin was sutured and sterilized with physiological saline. In the PI3K group, PI3K inhibitor LY294002 solution was administered 20 minutes before VD establishment. The operation in the sham group was identical to that mentioned above, without ligation. All rats maintained a body temperature of 37 ∘ C during anesthesia. After consciousness, the rats were housed at room temperature. Penicillin was intraperitoneally injected for two consecutive days to prevent infection.
Six weeks after surgery, the behavioral symptoms of rats were observed, neurological function scores were performed, and the cognitive ability and memory ability of each group were evaluated by water maze. After the experiment, the blood was collected by Orbital Blood collection and centrifuged to get serum. The brain tissue of each group was taken out. Half of the brain tissue was fixed in 4% paraformaldehyde, and the other half of the brain tissue was removed. To obtain the white matter, the rat's brain was cut into 2mm thick cerebral coronal slices. A thin white structure between the cortex and the deep brain tissue (such as the hippocampus) was observed, which was the cerebral white matter, then separated with a scalpel, cooled on the ice, and stored at -80 ∘ C.

Dosage and Method of Administration.
In the PI3K group, after anesthesia, the head was fixed with a stereotactic instrument. Stereotaxic location on the lateral ventricle: a hole was drilled with a dental drill 0.9 mm lateral and 1.5 mm posterior to Bregma, at the depth of 3.8 mm. 10 l 10 mmol/L LY294002 solution was slowly injected with a microsyringe within 5 minutes. The microsyringe was maintained in place for 5 minutes and then slowly withdrawn. Make sure to observe that there is no blood, no liquid medicine, or no cerebrospinal fluid overflow at the puncture point after needle extraction, the scalp was sutured, and the puncture was completed. In the LNMT and HNMT groups, according to previous experimental animal studies, the rats were intragastrically administered 0.56g/kg and 2.24g/kg NMT, respectively [20]. The same batch (Batch No. 2018010) of Naomaitai Capsule was used in this study to ensure a stable therapeutic effect. Naomaitai powder was dissolved in double distilled water and heated in a water bath at 37 ∘ C, vortex to a suspension of powder evenly dispersed. The rats in the PI3K group were treated with the dose of HNMT group. NMT administrate once 2mL a day for 5 days and operation 2 days after discontinuation of medication. In the model and sham groups, the equivalent amount of double distilled water was used as a placebo during the treatment.

Neurological Deficit
Score. Bederson scoring system was used to detect neurological impairment in rats. At 6 weeks after surgery, a single blind method was used to score neurological symptoms (that is, observers did not know the way of group assignment). Using the Bederson neurological deficit score method as a standard, the symptoms of each group of rats were observed; the neurological function of the rats was scored; and the symptoms of neurological deficit were recorded [21]. The scoring criteria are as follows: score 0: no symptoms of nerve damage; score 1: the contralateral forelimb cannot be fully extended when lifting the tail; score 2: turn to the temporal side while walking; score 3: fall to the opposite side of the lesion; score 4: cannot walk spontaneously.

Morris Water Maze
Test. The Morris water maze consists of a circular pool of 1.5 m diameter, a camera directly above the pool, and a computer program connected to the camera.
Evidence-Based Complementary and Alternative Medicine 3 Forced swimming: The navigation test was conducted to observe the time spent in the target quadrant for 5 days of training. After 5 days of training, the platform was removed from the water. The spatial probe test was performed to observe the number of platform location crosses so as to measure cognitive and memory abilities. At 6 weeks after surgery, Morris water maze test was carried out to assess the cognitive and memory abilities in VD rats.
2.6. HE Staining. At 6 weeks after model establishment, five rats from each group were obtained for HE staining in rats; the samples were obtained. After decapitation, the white matter was gained, fixed in 10% paraformaldehyde for 48 hours, dehydrated, permeabilized, embedded in wax, and sliced into sections. The sections were stained with hematoxylin and eosin. The histopathological changes of cerebral white matter were observed under a light microscope.

TUNEL Assay for Neuronal Cells in the White Matter.
TUNEL Kit (No. 11684817910, Roche, USA) was used to detect the apoptosis of white matter neurons according to the detailed instructions. The white matter fixed in paraformaldehyde was dehydrated, embedded, and sliced. The sections were incubated with 0.9% NaCl for 5 minutes and washed twice with PBS. After pouring out the liquid, biotinylated nucleotides and terminal deoxynucleotidyl transferase (1:500 dilution) were added and mixed well. After covering plastic cover glass, the mixture was incubated for 60 minutes at 37 ∘ C, washed with PBS, and treated with 0.3% H 2 O 2 . After three washes with PBS, horseradish peroxidase-(HRP-) labeled streptavidin was added and incubated for 30 minutes at room temperature, followed by PBS washes. The sample was observed and photographed with a microscope.

ELISA for MDA and SOD Contents as Well as S-100 and NSE Contents in Brain.
Oxidative stress factor and brain damage markers contents in white matter were determined by ELISA. ELISA kit was used to detect the contents of white matter oxidative stress factors MDA (CEA597Ge, uscn, USA) and SOD (SES134Ra, uscn, USA) as well as white matter damage markers S-100 (SEA567Ra, uscn, USA) and NSE (SEA537Ra, Uscn, USA) contents according to the instructions. 100 ul standard preparation and l00 ul diluted sample were added to the corresponding reaction plate well, mixed, and incubated at 37 ∘ C for 30 minutes. After the plate was washed, 100 ul tested sample was added in each well and incubated for 2 hours at 37 ∘ C. After the plate was washed, l00 ul HRP-labeled secondary antibody was added and incubated for 30 minutes at 37 ∘ C. After the plate was washed, the samples were visualized by adding 50 ul coloring solution A and coloring solution B in the dark for 15 minutes. The reaction was terminated by adding 50 ul stop buffer. Optical density (OD) values were read at 450 nm using the microplate reader (EXL808, USA). The standard curves were drawn. The corresponding concentration of the sample was calculated according to the curve equation.

Western Blot Assay to Detect Related Protein Expression.
The protein expression of PI3K/PDK1/AKT signaling pathway-related proteins, apoptosis-related proteins were detected by Western blot.
Through after frozen white matter was added to the precooling tissue protein lysate, homogenate suspension was made by tissue homogenizer. Protein content was detected in BCA protein detection kit. The protein concentration was adjusted for SDS-polyacrylamide gel electrophoresis, and the proteins were transferred onto the membrane using a Trans-Blot transfer system (1703930, BIO-RAD, USA). The membrane was blocked with confining liquid for 2 hours. PI3K (ab151549, Abcam, USA), PDK1 (ab110025, Abcam, USA), AKT (ab8805, Abcam, USA), Bcl-2 (ab59348, Abcam, USA), Caspase3 (ab13847, Abcam, USA), and Bax (ab32503,Abcam, USA) primary antibodies were added and incubated at 4 ∘ C overnight. After three washes with TBST, secondary antibodies were added and incubated for 1 hour, followed by four washes with TBST. The sample was visualized with ECL luminescent kit (35050, Pierce, USA) and imaged with the gel imaging system. The gray value was analyzed by Quantity One software.

Detection of White Matter Nerve Fiber Damage by LFB
Staining. The brain tissue sections of each group were taken. Three sections were taken from each rat. After dewaxing, the sections were put into LFB staining solution, sealed and immersed for 24 hours at 60 ∘ C, Washed with distilled water and 95% ethanol. After separating the color with a 0.05% lithium carbonate aqueous solution, the color separation was continued with 70% alcohol until the gray and white matter were clearly observed under the microscope. The gray matter is transparent and the white matter is blue. After being dehydrated by alcohol gradient, samples were transparent twice by xylene and sealed by the neutral gum was. The damage of the white matter nerve fibers was observed under microscope.
2.11. Immunofluorescence for the Expression of PI3K, PDK1, AKT and MBP at the White Matter. Paraffin sections were dewaxed, hydrated, immersed in 3% hydrogen peroxide solution for 15 minutes, and washed with PBS. Antigens were retrieved with 0.1 M sodium citrate. The sections were blocked with goat serum and incubated for 30 minutes at 37 ∘ C. After removal of serum, without washing, PI3K (ab151549, Abcam, USA), PDK1 (ab110025, Abcam, USA), AKT (ab8805, Abcam, USA), and MBP (ab40390, Abcam, USA) antibodies were added and incubated at 4 ∘ C overnight. The sections were washed with PBS and incubated with fluorescence-labeled secondary antibody for 30 minutes at 37 ∘ C, followed by PBS washes. DAPI-stained nuclei were added and incubated at room temperature for 10 minutes, followed by PBS washes. The sections were mounted with neutral resin and observed with a fluorescence microscope. analyzed using SPSS 19.0 software and expressed as the mean ± standard deviation. Intergroup comparison was carried out with one-way analysis of variance. Intragroup comparison was conducted using repeated measures analysis of variance. A value of P < 0.05 was considered statistically significant.

NMT Ameliorated Neurological Impairment in VD Rats.
Afterbilateral common carotid arteryocclusion, compared with the sham group (0±0) in the VD group the neurological deficit score increased (3.38±0.39) and spatial cognitive ability and spatial memory ability were poor (P < 0.05). After NMT treatment, the neurological deficit score decreased and spatial cognitive ability and spatial memory ability were effectively improved in VD rats. Nevertheless, neurological deficit score results were not significantly different between the HNMT (1.86±0.22) and the LNMT (1.97±0.11) groups ( Figure 1(a)). After 5 days of training, it demonstrated that the latency in the navigation test was long in VD rats. In the spatial probe test, VD rats showed nondirectional trajectory in the pool. Compared with the sham group (the time spent in the target quadrant, 5.62±0.58; the number of platform location crosses, 9.65±0.84), the time in the target quadrant (1.61±0.49) and the number of platform location crosses (2.6±0.77) were significantly reduced (P < 0.05). After NMT treatment, rats swam in the pool under the same conditions in the HNMT and LNMT groups. The navigation test and spatial probe test results demonstrated that the latency finding the platform was remarkably shortened, and the behavior of the rats was purposeful after removing the platform. The time in the target quadrant (HNMT, 3.22±0.72; LNMT, 3.18±0.66) and the number of platform location crosses (HNMT, 7.66±0.63; LNMT, 7.52±0.51) were obviously increased (vs. VD, P < 0.05) (Figure 1(b)). The results indicated that NMT has a therapeutic effect on neurological deficit rats, and the therapeutic effect is not associated with the dosage.

NMT Improves White Matter Damage in VD Rats.
HE staining result showed that the structure of brain was normal, the fibers of the corpus callosum were arranged and there was no obvious vacuolar structure in the Sham group. In the VD group, the white matter was damaged, the fibers of the corpus callosum were disordered, and a large number of vacuolar structures were observed. Elisa showed that S-100 and NSE contents markedly increased in the VD group (S-100 , 1.42±0.09; NSE, 4.19±0.59; P < 0.05) compared with the sham group (S-100 , 0.67±0.09; NSE, 2.18±0.61). In the HNMT and LNMT groups, the fibers of the corpus callosum are arranged and only a few vacuoles appeared in the white matter. S-100 (HNMT, 0.74±0.07; LNMT, 0.77±0.09) and NSE (HNMT, 2.56±0.44; LNMT, 2.62±0.62) contents diminished (vs. VD, P < 0.05). There were no significant differences between the HNMT and the LNMT groups ( Figure 2). These findings indicated that NMT can repair the white matter damage in VD rats.  (Figure 3(a)). These results indicated that NMT inhibits white matter oxidative stress and improves white matter damage.  (Figure 3(b)). These findings confirmed that NMT achieves the therapeutic effect by inhibiting the expression of inflammatory factors. sheath, LFB staining was performed. It showed in sham group the myelin sheath fibers in the corpus callosum were arranged neatly and compactly, oligodendrocyte structure was intact, no vacuole structure. In VD group, the gap between myelin sheaths became larger, and a large number of vacuoles were observed due to oligodendrocyte decreasing, Myelin arrangement is irregular, more chaotic, and the staining is obviously lighter (vs. sham), which were typical demyelinating lesions appeared in corpus callosum. After administration of Naomaitai, the myelin sheath in LNMT group was denser and the disordered arrangement was improved. The staining degree of LFB was significantly higher than that in VD group.

Evidence-Based Complementary and Alternative
There was no significant difference between HNMT group and LNMT group (Figure 4(a)). MBP is the basic protein in myelin sheath. The MBP in white matter of rats in each group was observed by IF. The results showed that the MBP in the sham operation group was higher. However, in VD group, white matter damage was caused by chronic white matter deficiency, and MBP expression decreased (vs. sham, P<0.05). After Naomaitai administrated, the expression of MBP in white matter of rats in HNMT group and LNMT group increased (vs. VD, P < 0.01). There was no significant difference in protein expression between the two treatment groups (P>0.05) (Figure 4(b)). The results suggested that Naomaitai can improve the low expression of MBP caused by myelin sheath injury, reduce the damage and loss of myelin sheath caused by insufficient cerebral perfusion, and play a protective role in white matter.

NMT Inhibits Apoptotic Factor Expression in the White
Matter of VD Rats. TUNEL assay ( Figure 5(a)) and western blot assay ( Figure 5(b)) showed that white matter neurons had obvious apoptosis compared with sham group (apoptotic rate, 3.31±0.52), and apoptotic rate remarkably increased in the VD group (apoptotic rate, 42.82±6.22). Apoptosis-related protein expression data demonstrated that Bcl-2 expression reduced, caspase-3 and Bax expression increased in the VD group (vs. Sham, P < 0.05). The apoptotic rate decreased; but Bcl-2 expression increased; and caspase-3 and Bax expression reduced in the HNMT (apoptotic rate, 19.42±1.49) and LNMT (apoptotic rate, 21.35±2.52) groups (vs. VD, P < 0.05). The results suggested that NMT plays an antiapoptotic role in the VD model.

NMT Mitigates Brain Injury in VD Rats through the PI3K/ PDK1/AKT Signaling Pathway.
Immunofluorescence method (Figures 6(a)-6(c)) and western blot assay ( Figure 6(d)) were used to determine the protein expression of PI3K, PDK1, and AKT. The results revealed that PI3K, PDK1, and AKT expression increased in the white matter after model establishment in the VD group (vs. Sham, P < 0.05). After NMT treatment, PI3K, PDK1, and AKT expression decreased in the white matter in the HNMT and LNMT groups (vs. VD, P < 0.05). Our results indicated that NMT could ameliorate hypoxia and ischemia in the white matter of VD rats, and the therapeutic effect may be associated with the inhibition of expression of the PI3K/PDK1/AKT signaling pathway.

Discussion
This study identified that NMT had a significant effect on improving neurological impairment and alleviating ischemia and hypoxia in VD rats. Simultaneously, NMT could also achieve the therapeutic effect of inhibiting oxidative stress, reducing white matter-related apoptosis protein and PI3K/PDK1/AKT signaling pathway protein expression. These results suggested that NMT has protective effects on white matter of VD rats, which may be achieved by regulating PI3K/PDK1/AKT signaling pathway.
VD is a common disease in the elderly population, and is an age-related cognitive disorder [22]. A large amount of data showed that most patients with dementia presented different degrees of white matter damage [23]. We infer that the key factors affecting cognitive ability are white matter damage, inflammation in the central nervous system, oxidative stress and neuronal apoptosis caused by long-term hypoxia and hypoperfusion, which are also the main causes of white matter damage. Therefore, strengthening the protection of white matter and reducing neuronal apoptosis are key issues in the treatment of VD [24].
Excitatory amino acid toxicity, free radicals and NOinduced oxidative stress injury and inflammatory reaction are the main factors that mediate neuronal apoptosis after cerebral ischemia [25][26][27]. Apoptosis is the phenomenon of programmed cell death under gene regulation [28]. Bcl-2 encoded by Bcl-2 proto oncogene plays an important role in promoting cell survival and apoptosis [29]. Activation of a series of downstream genes of pro-apoptotic factor Bax can accelerate cell apoptosis [30]. Caspase is an aspartatespecific protease and a major performer of apoptosis [31]. Caspase-3 is the most important apoptotic factor in the caspase apoptotic pathway [32]. PI3K/PDK1/AKT signaling pathway is the key signal transduction pathway to inhibit cell apoptosis in cells [33]. Because of PI3K activation stimulated by external stimuli, phosphatidylinositol phosphorylation is catalyzed to produce the second messenger: inositol [34]. Under the control of inositol, AKT is transferred from cytoplasm to cell membrane, and is phosphorylated by PDK1 assisted AKT protein threonine site [35]. The active AKT after phosphorylation regulates the related expression of downstream apoptotic factors and inhibits apoptosis [36].  Figure 7: PI3K inhibitor reverses the therapeutic effect of NMT on VD rats. Bederson scoring system was used to detect neurological impairment in rats. MWM test was conducted to determine the spatial cognition and memory ability of rats. HE staining was utilized to observe the changes of brain tissue morphology in rats. ELISA was performed to determine the expression levels of brain damage markers, oxidative stress factors and inflammation related factors. Apoptosis-positive cells were determined via Tunel assays. Apoptosis-related protein expression was determined via Western blot assay. Immunofluorescence method and western blot assay were used to determine the protein expression of PI3K, PDK1, and AKT. LFB staining was utilized to observe the damage of white matter nerve fibers and the loss of myelin sheath. Immunofluorescence method was used to determine the MBP expression in white matter of rats. Previous studies have found that many traditional Chinese medicines have therapeutically effect on VD [37][38][39][40]. Zhu et al. have found that Panax ginseng extract is neuroprotective against vascular dementia induced by chronic cerebral hypoperfusion [37]. Fan et al. have identified that moxibustion intervention is able to improve the delayed memory in VD rats [38]. NMT capsule takes ginseng and Sanchi as principal drugs, which can invigorate vital energy, produce blood, dissipate blood stasis, and promote blood circulation [41]. NMT capsule takes Chinese Angelica, ginkgo leaf, and Danshen Root as ministerial drugs, which can clear and activate the channels and collaterals [8]. As the remarkable effects of supplementing Qi, activating blood circulation, removing blood stasis, dredging collaterals, expelling wind, and eliminating phlegm, NMT capsule is clinically used in the recovery phase of ischemic stroke [10,11]. Previous studies showed that NMT has therapeutic effect on VD [20,42,43] and the specific mechanism of the protective effect has not been reported. Ischemic stroke is equivalent to acute ischemic cerebrovascular disease such as cerebral infarction in western medicine [44]. Therefore, we can conclude that NMT capsule can improve cerebral hypoperfusion in the brain of rats. NMT has been shown to reduce the occurrence of cognitive impairment by improving the cerebral ischemia Evidence-Based Complementary and Alternative Medicine 15 and hypoxia in VD rats and protecting the white matter [8].
It was shown that, after bilateral common carotid arteryocclusion 6 weeks, rats not only showed behavioral disorders but long-term hypoperfusion activated cells in the white matter, which in turn led to proliferative lesions, enlarged cell bodies, and many neurites and mediated the inflammatory response by secreting a series of active substances [45]. White matter damage caused by long-term hypoxia and hypoperfusion can cause cognitive decline, oxidative stress during cerebral ischemia, and excessive free radical [46]. Although there are few studies on the detection of oxidative stress markers in VD, some data support the existence of oxidative stress in VD [47,48]. Sinclair et al. [49] pointed out that the level of antioxidant trace element vitamin C decreased in plasma of VD. Furthermore, Casado et al. [50] proved that malondialdehyde levels were higher in VD patients compared with the control group. 8-Hydroxy-2 deoxyguanosine (8-OHDG) contents obviously increased in the cerebrospinal fluid and urine of VD patients [51]. These studies showed that oxidative stress levels are altered in VD. Cerebral autosomal dominant arteriopathy with subcortical infarcts and leukoencephalopathy(CADASIL) is a type of VD [52]. The studies have found that there is extensive neuronal apoptosis in the brain of CADASIL patients, and the occurrence of apoptosis is due to hypoxia and hypoperfusion injury in the brain [53]. Further research on the apoptotic pathway is expected to provide new treatments for VD. Therefore, this study examined inflammatory factors, oxidative stress factors and apoptotic factors in VD model rats. The results showed that NMT can inhibit the occurrence of inflammatory response, oxidative stress and apoptosis. The results suggested that the protective effect of NMT may be associated with its inhibition of white matter inflammatory reaction, peroxidation and apoptosis.
The PI3K/PDK1/AKT signaling pathway plays an important role in the regulation of cell proliferation, and its main signaling molecules include PI3K, PDK1 and AKT [54]. Activation of PI3K activates downstream protein kinases, PDK1, and AKT and both PDK1 and Akt contain a PH domain [55]. This domain binds to PI(3,4,5)P3, translocating them to the plasma membrane of the cell and phosphorylation of PDKI activates AKT. Activated AKT phosphorylates Bax and inhibits the formation of dimers between Bax and Bcl-2 [56]. Dissociated Bcl-2 plays a key role in inhibiting apoptosis [57]. PDK1 is a downstream protein of PI3K and plays an important role in physiological processes such as cell metabolism, growth and survival [58]. Cellular assay results show that PDK1 loss leads to a large number of apoptosis; and a major network composed of Cyclin, cyclin-dependent protein kinase (CDK), and CDK inhibitory protein (CKIs) can coordinate the regulation of the cell cycle [59]. In the present study, a VD rat model was established and was given different doses of NMT simultaneously. Then, the PI3K antagonist LY294002 was injected into the brain. Our results indicate that NMT can inhibit neuronal apoptosis, increase Bcl-2 expression, decrease caspase-3 and Bax expression, and downregulate the expression of PI3K, PDK1, AKT, and P-AKT. However, these changes can be reversed by LY294002.
The results indicated that NMT may improve neuronal apoptosis in VD rats through PI3K/PDK1/AKT pathway, and the activation of PI3K/PDK1/AKT signaling pathway may be an important method for the treatment of cognitive decline.
This study explored the therapeutic effect of naomaitai on VD rats, providing a new idea for VD treatment. However, the specific components of naomaitai that play a protective role were not discussed, and the analysis of the specific components that have an effect could provide a more perfect strategy for VD treatment.

Conclusions
Naomaitai can ameliorate brain damage in rats with vascular dementia, inhibit neuronal apoptosis, and have antiinflammatory and antioxidative stress effects, which may be regulated by the PI3K/PDK1/AKT signaling pathway.

Data Availability
The data used to support the findings of this study are available from the corresponding author upon request.