Creating a mouse model resistant to induced ischemic stroke and cardiovascular damage

Vascular prostanoids, isomerized from an intermediate prostaglandin (PG), H2, produced by cyclooxygenase (COX), exert various effects on the vascular system, both protective and destructive. During endothelial dysfunction, vascular protector prostacyclin/prostaglandin I2 (PGI2) is decreased, while inflammatory PGE2 and thrombotic TXA2 are increased. Therefore, our research aim was to reverse the event by controlling PGH2 metabolism by generating an in vivo model via enzymatic engineering of COX-1 and prostacyclin synthase (PGIS). The COX-1 and PGIS genes were linked to a 10-residue amino acid linker to form a Single-chain Enzyme Complex (SCHEC), COX-1-10aa-PGIS. Transgenic (CP-Tg) mice in a FVB/N background were generated using the pronuclear microinjection method. We first confirmed mRNA and protein expression of COX-1-10aa-PGIS in various CP-Tg mouse tissues, as well as upregulation of circulating PGI2. We then examined the cardiovascular function of these mice. Our CP-Tg mice exhibited marked resistance to vascular assault through induced carotid arterial blockage, acute thrombotic stroke and arterial arrest, angiotensin-induced peripheral vasoconstriction, and hepatic lipid accumulation after receiving a high-fat diet. They also had a longer lifespan compared with wild-type mice. This study raises the possibility of fighting cardiovascular diseases by regulating cellular arachidonic acid-derived PGH2 metabolites using enzymatic engineering.

associated with the prevention of its conversion to thrombotic TXA 2 and inflammatory PGE 2 , could provide a fundamental approach to restore endothelial dysfunction for the prevention and treatment of cardiovascular diseases. To achieve this goal, we recently employed an enzyme clustering method, in which we channeled PGH 2 by linking COX-1 enzyme and PGIS enzyme to a well-defined 10-residue amino acid linker 10 . With the enzyme complex, we were able to regulate prostanoid biosynthesis in favor of PGI 2 rather than TXA 2 and PGE 2 in cells. The varied cells, including COS-7, HEK293 11,12 , primary cultured adipose stromal cells 13 and endothelial progenitor cells 14 , were transfected with the single cDNA of COX-1-10aa-PGIS or COX-2-10aa-PGIS. They showed high expression levels of the active hybrid enzyme with triple catalytic activities (converting AA into PGG 2 , then PGH 2 and finally into active PGI 2 ), which resulted in redirecting the conversion of endogenous AA metabolites more toward the favorable PGI 2 production rather than the unfavorable TXA 2 and PGE 2 production [11][12][13] . These in vitro molecular and cellular studies, and preliminary experiments 15 have provided a basis for us to hypothesize that the single gene of the hybrid enzyme could reduce the risk of heart disease in vivo. In this study, we integrated the protein engineering, enzyme complex construction, and transgenic mouse technique to gain primary control of cellular AA metabolism in favor of PGI 2 biosynthesis and to disfavor PGE 2 and TXA 2 biosynthesis in vivo. The study was proposed in a previous editorial paper 15 . Here, with comprehensive experiments and more data, we demonstrated that the transgenic mouse model exhibited marked resistance to vascular assault through induced carotid arterial blockage, induced acute thrombotic stroke and arterial arrest, and angiotensin-induced peripheral vasoconstriction. The safety of the engineered trans-gene, COX-1-10aa-PGIS (integrated COX-1 and PGIS activities together in a single polypeptide chain) was confirmed by healthy animal development and maintenance of a longer lifespan with improved mental performance, which has been demonstrated in a previous publication 16 . It greatly increased the possibility of correcting inherited heart diseases using emerging gene medicine, such as the transgene, COX-1-10aa-PGIS, at the current experimental level.

Results
Generation of transgenic mice carrying a SCHEC, COX-1-10aa-PGIS gene. We first demonstrated that the microenvironment of cellular prostanoid biosynthesis in primary cells could be controlled by our SCHEC, COX-1-10aa-PGIS (Fig. 1ia). Arachidonic acid metabolism was redirected in favor of PGI 2 biosynthesis and disfavor to inflammatory PGE 2 and thrombotic TXA 2 biosynthesis for vascular protection, which was demonstrated in vitro and in vivo in our previous publication 15 . These data led to the hypothesis that the symptoms of cardiovascular diseases could be reduced by expression of a single gene, COX-1-10aa-PGIS, in vivo. To test this hypothesis, the COX-1-10aa-PGIS cDNA with a pCMV promoter for general expression and a pA segment were isolated from the COX-1-10aa-PGIS pcDNA3.1 vector (Fig. 1ib). Next, the founders of the original pair of COX-1-10aa-PGIS transgenic mice (CP-Tg mouse/mice) were created by pronuclear microinjection technology using the isolated COX-1-10aa-PGIS cDNA ( Supplementary Fig. 1).
Identification of the CP-Tg mice permanently incorporated with the single gene of COX-1-10aa-PGIS. A special set of polymerase chain reaction (PCR) primers was designed to determine the presence of the human COX-1-10aa-PGIS gene in the CP-Tg mouse chromosome. The primers contained the 3′-and 5′-ends of a unique DNA sequence of the center region of the incorporated single gene of COX-1-10aa-PGIS (from the C-terminal domain of COX-1 to the 10-aa linker and the N-terminal domain of PGIS) comprising a total of 445 bp (Fig. 1iia). Of the first 29 newborns, three founders (Fig. 1iib, lanes: 3, 11 and 26) permanently carrying the COX-1-10aa-PGIS gene were identified from mouse tail DNA by the tail cut-PCR approach using the designed primers. The founders were further bred with wild-type FVB/N mice and found to pass the transgene following Mendelian rules. The resulting seven heterozygous mice were further identified by the tail cut PCR approach (Fig. 1iic, lanes 3, 4, 6, 8, 9 and 10).
The gene profile of COX-1-10aa-PGIS expression in different organs. The expression of individual COX-1 and PGIS were tissue-specific. COX-1 was relatively widely expressed, but PGIS was largely localized in vascular endothelial cells and smooth cells. It was of interest to observe the tissue specificities of the hybrid gene and protein after combining COX-1 and PGIS in one molecule using the pCMV promotor for general expression. Therefore, to evaluate anatomical changes in CP-Tg mice, the major organs were isolated: heart, lung, kidney, brain, and liver. The distribution of the COX-1-10aa-PGIS gene in different tissues of CP-Tg mice was identified by PCR using specific primers as described above. Figure 2a shows the permanent distribution of the COX-1-10aa-PGIS gene according to the different organs. Importantly, the gene was detected in the heart, kidney, and brain, each of which benefitted from the vascular protection provided by the hybrid enzyme. The protein expression of COX-1-10aa-PGIS enzyme in major organs was further identified by Western blot analysis (Fig. 2b). It should be noted that COX-1-10aa-PGIS has a unique molecular mass, 130 kDa, which could be easily distinguished from endogenous COX-1 and PGIS. Similar to the gene distribution profile, COX-1-10aa-PGIS protein was expressed in the major organs: heart, lungs, brain, and kidneys. This result suggested that the single active COX-1-10-aa-PGIS gene could be a potential protector against ischemic heart disease, kidney failure, and stroke caused by thrombosis and vasoconstriction. However, none of the organs showed any gross anatomical difference as observed in CP-Tg mice ( Supplementary Fig. 3). Additionally, we also examined the gene and protein expression of COX-1-10aa-PGIS in other organs, except for those major ones. The gene expression was detected in all other organs, and most organs also expressed the protein, except pancreases. Together, these data suggested that our hybrid enzyme COX-1-10aa-PGIS had been successfully integrated into the mice.  The sequence of COX-1 linked to PGIS through a 10-aa linker (COX-1-10aa-PGIS) was generated by PCR and subcloning procedures by the vector company (Invitrogen). The resulting cDNA was successfully subcloned into the pcDNA 3.1 vectors at Kpnl and BamHl sites containing a cytomegalovirus early promoter by PCR. The cDNA fragment (3.2 kb) containing COX-1-10aa-PGIS, a pCMV promoter and a PGH polyadenylation site (pA) was cut at the Nrul and Sphl sites from the COX-1-10aa-PGIS-pcDNA3.1 vector and purified to a single band as a transgenic gene for preparation of the transgenic mice. (iia) PCR primers designed to examine integration of the gene, a unique DNA fragment of 445 bp, into the genome. (iib) Genotyping of the first founders of the transgenic mice by PCR. The incorporated DNA of COX-1-10aa-PGIS in the mice was determined by PCR using the primers described in (iia), mouse tail tissues as template, and analysis by agarose gel electrophoresis to identify the specific 445-bp hybrid enzyme. (iic) PCR analysis of the second group of transgenic mice using the tail cut PCR approach in an identical manner to the procedures described in the (iib) panel.
SCiEnTifiC REPORTS | (2018) 8:1653 | DOI:10.1038/s41598-018-19661-y MS analysis. The ratio of the metabolites of AA to PGI 2 (final inactive product is 6-keto-PGF 1α ) to PGE 2 and TXB 2 (inactive metabolite of TXA 2 ) was 7 in the CP-Tg mice and 1 in the wild-type mice (Fig. 2c,d). We also showed the amount of 6-keto-PGF 1α , TXB 2 , and PGE 2 in 24 h urine (Fig. 2e) 4. The results revealed that the incorporated COX-1-10aa-PGIS gene into mice exerted multiple effects on the vascular circulation in vivo: a) increased PGI 2 biosynthesis, b) reduced thrombotic TXA 2 production, and c) decreased inflammatory PGE 2 biosynthesis. This triple effect could result in a synergetic vascular protection against thrombotic and vasoconstrictive damages from heart diseases in vivo. Identification of the vascular protective potential through anti-coagulation/anti-thrombosis activity of the single COX-1-10aa-PGIS gene in transgenic mice. One of the major vascular protective characteristics of increased PGI 2 with decreased TXA 2 is anti-coagulation/anti-thrombosis. Thus, bleeding time was used as an indication to detect the vascular protective potential of the COX-1-10aa-PGIS gene in the transgenic compared with normal WT mice. Supplementary Fig. 4 shows a representative picture of how the bleeding time was measured using filter paper, which is described in Material and Methods. The bleeding time was 55 mins (n = 6) for CP-Tg mice, which was 3.7-fold longer than that of wild-type mice with an average bleeding time of 15 mins (Fig. 3a). However, no blood cells or oxidized hemoglobin were found in the urine and stool of CP-Tg mice, which indicated bleeding tendencies in the gastric system, intestinal system, and urinary tract were unlikely in the CP-Tg mice. Another possible change caused by the up-regulated PGI 2 production may be reduced blood pressure. This was not the case for the CP-Tg mice. Their blood pressure, both systolic and diastolic ( Fig. 3b), along with heart rate measurement ( Fig. 3c) of both TG(+/+) and WT mice, showed no significant differences. In addition, blood counts, cholesterol, and glucose levels were within the normal ranges observed in wild type (data not shown).
CP-Tg mouse resistance to the induced thrombotic reaction using carotid artery thrombosis as a model. The vascular protective effect on vascular disease caused by permanent COX-1-10aa-PGIS gene expression was demonstrated in a carotid artery thrombosis model. Using this model, both CP-Tg and WT mice were tested for resistance to thrombosis, one of the major leading causes of stroke and heart arrest. The thrombotic obstacle of the carotid artery was induced by photothrombotic ischemia using the combination of Rose Bengal injection, followed by a laser beam light targeting the local artery. Typical real-time monitoring of the blood flow in the occluded carotid arteries of wild-type (Fig. 4a, top panel) and CP-Tg (Fig. 4a, lower panel) mice are shown. The blood flow was not reversibly shut down within 5 minutes, leading to death within a couple hours in wild-type mice (Fig. 4a, top panel). By contrast, blood flow, which was reduced to 90% at the beginning of the induced thrombosis in the artery, quickly recovered to 50% within a few minutes, and then to 70, 80, and 90% within a couple hours in CP-Tg mice (Fig. 4a, bottom panel), which survived the procedure. Further studies with 10 animals in each group provided consistent results (Fig. 4b). The average induced thrombosis in the carotid artery associated reduced blood flow started within minutes and progressed within 2 hours in wild-type mice ( Fig. 4b red squares, n = 10). However, in CP-Tg mice, the decreased blood flow during the first few minutes was reversed to 80% normal flow at 20 minutes, and completely recovered after 2 hours, avoiding animal death (Fig. 4b, black squares). These results suggested that CP-Tg mice resisted thrombotic stroke and death induced by Rose Bengal/laser-induced carotid artery thrombosis.
CP-Tg mouse resistance to death by AA-induced stroke and cardiac arrest. An additional thrombotic stroke model was created by overproducing TXA 2 in the circulation using intravenous (IV) injection of the TXA 2 precursor AA (Fig. 5a). Due to the enrichment for COX-1 and TXA 2 synthases in platelets, the infused AA (from IV) could quickly lead to enhanced synthesis of TXA 2 and trigger platelet aggregation and vasoconstriction, which could a) immediately induce reduced blood circulation in the brain and cause stroke; and/or b) block the coronary artery blood supply and cause cardiac arrest. All wild-type mice suffered from thrombotic stroke and heart arrest after infusion of an average of 10 mg/kg of AA (LD50 = 5 mg/kg, Fig. 5b) within 30 minutes. However, thrombotic stroke and cardiac arrest leading to death was dramatically delayed in CP-Tg mice until they were given an average of 100 mg/kg of AA (LD50 = 50 mg, Fig. 5b). To evaluate the resistance of CP-Tg mice Blood pressure measurement by the tail cutting method. Both systolic and diastolic blood pressure was measured in TG and WT mice. (c) Heart rate measurement by the tail cuff method. Heart rate was measured along with blood pressure in both TG and wild-type mice. The values shown are the mean ± SD (n = 7, p < 0.001). The data were analyzed by the student's t-test.
SCiEnTifiC REPORTS | (2018) 8:1653 | DOI:10.1038/s41598-018-19661-y to the induced stroke, a time course of reperfusions of AA-induced ischemia and stroke was monitored using a laser Doppler image system (Fig. 5c). The CP-Tg mice showed initial ischemia for the first 10 minutes, followed by rapidly reperfusion to almost normal blood flow at 25-30 mins during AA (10 mg/kg) induction (Fig. 5c). By contrast, wild-type mice suffered from AA-induced ischemia and were unable to perform the reperfusion, leading to permanent ischemia and death (Fig. 5c). Quantitative data of the integrated intensity are displayed in Fig. 5d. Similarly, the brain anatomy also confirmed that the CP Tg-mice maintained normal blood reperfusion and did not develop vascular damage under 10 mg/kg AA induction at the end of the experiment (2 hours). However, ischemic and vascular damage were clearly observed in wild-type mice under identical conditions ( Supplementary Fig. 5). Our results indicated a remarkable protection against stroke and cardiac arrest by the permanently incorporated single hybrid enzyme gene in transgenic mice.

CP-Tg mice are resistant to non-prostanoid-related vasoconstrictive damage.
To evaluate the resistance of CP-Tg mice to any non-prostanoid-related vascular damage, angiotensin-induced vasoconstrictive ischemia was used. In general, angiotensin can cause vascular stress by inducing acute vascular constriction, which results in reduced blood flow in peripheral and major organs, such as brain, heart, and kidneys. The changes in peripheral blood reperfusion in the hind limbs of mice were monitored by laser Doppler scanning before and after administering angiotensin to the animals. CP-Tg mouse resistance to induced vasoconstrictive ischemia was clearly observed (Fig. 6). All three CP-Tg mice showed slightly decreased reperfusion from 2-15 minutes, followed by recovery to almost normal reperfusion at 30 minutes after receiving the angiotensin (Fig. 6a). In comparison, the reperfusion of all three wild-type mice was dramatically reduced starting at the first minute up to the thirtieth minute without recovery after angiotensin injection (Fig. 6b). These results indicated that the incorporated COX-1-10aa-PGIS gene in transgenic animals was able to resist the induced vascular damage.
CP-Tg mice are resistant to high-fat diet-induced lipid accumulation. A high-fat diet was fed to the CP-Tg and wild-type mice for 6 months. Anatomic analyses were performed to compare lipid accumulation in liver. Figure 7a shows much less lipid accumulation in the liver of CP-Tg compared with wild-type mice. We used particle analysis in ImageJ to examine the lipid accumulation in liver, in which the dark spots represent lipid accumulation. The count is the number of dark spots, while the total area and the % area indicate the intensity of the dark spots. Additionally, the average size indicates the average particle size, and the mean is the mean intensity of the entire image. Because of the similar average particle size and image background, the lower total area and % area observed in our Tg mice after a high-fat diet suggested a reduction of hepatic lipid accumulation. These data further indicated that the controlled AA metabolites favoring PGIs and disfavoring PGE 2 and TXA 2 have beneficial resistance effects against high-fat diet-induced damage to the liver.

CP-Tg mice have a long lifespan.
The FVB/N CP-Tg mice and wild-type FVB/N-WT mice were maintained in identical life conditions, such as a stable temperature at approximately 24 °C with identical diets and general health care. Their overall lifespan was recorded for almost three years. The CP-Tg mice were not only free from suffering bleeding tendencies, headaches (no head-directed wiping and scratching 17 ), hypotension, and other vascular-related dysfunctions correlated with the progression of aging, but they also had longer lifespans in general (Fig. 7b), in which the longest life span reached almost 1000 days, with an average of 757.6 ± 40.63 days. Wild-type control mice had a longest lifespan of 670.5 ± 32.37 days (Fig. 7b).

Discussion
For decades, the use of PGI 2 mimic to treat vascular diseases, such as pulmonary arterial hypertension, has been well documented 18,19 . The vascular protective effects of PGI 2 have also been well demonstrated by studies showing an increase in the risk of heart attack associated with the use of COX-2 inhibitors, such as Vioxx, by suppressing PGI 2 production. By contrast, reducing TXA 2 production, such as through aspirin use, is a more traditional way to provide protection heart disease and stroke. Anti-inflammatory and anti-proliferation drugs are often used to treat vascular inflammation during restenosis and arteriosclerosis development through suppression of the biosynthesis of an inflammatory factor, such as PGE 2 . Thus, it becomes very interesting to develop an ideal intervention that could integrate the three forms, increasing PGI 2 biosynthesis associated with a decrease in TXA 2 and inflammatory PGE 2 production in vivo to enhance the protective power against heart disease and stroke. Our CP-Tg mouse is the first transgenic mouse line used to test this intervention. As expected, the single COX-1-10aa-PGIs gene incorporated into the mice redirected the endogenous AA metabolite in favor of PGI 2 production while reducing TXA 2 and PGE 2 in the circulation, as evidenced by LC/MS analysis (Fig. 3). In particular, functional COX-1-10aa-PGIS enhanced expression in major organs, such as the heart, brain, and kidneys, suggesting that the blood circulation and oxygen level might also be increased in these organs. This phenomenon could provide a fundamental benefit by preventing vascular diseases caused by acute thrombotic and vasoconstrictive damages, as well as chronic ischemia.
By contrast, there were no indications of any abnormal bleeding or hypotension, which might have resulted from the over-expression of COX-1-10aa-PGIS in transgenic mice. Although bleeding time was prolonged in CP-Tg mice due to the anti-thrombotic properties, it did not cause any bleeding disorders and remained within a safe range. PGI 2 is a potent endogenous vasodilator and may therefore lead to blood pressure lowering similar to the administration of a PGI 2 mimic. However, both the systolic and diastolic blood pressures of the CP-Tg mice were similar to those of wild-type mice using the tail cuff method (Fig. 5). This phenotype could be explained by compensatory mechanisms that regulate blood pressure to normal levels in CP-Tg mice, which is a common physiological effect when using the transgenic approach instead of drug therapy.
Thrombosis and vasoconstriction are major causes of death by stroke and cardiac arrest. The CP-Tg mice showed resistance to ischemia and death in the Rose Bengal/laser-and AA-induced thrombotic stroke and cardiac arrest models (Figs 4, 5), as well as resistance to angiotensin-induced vascular damage (Fig. 6). These data provide strong evidence that the single COX-1-10aa-PGIS gene has preventive and therapeutic value against thrombotic/vasoconstrictive heart disease and stroke in general.
Furthermore, it should be noted that a mental balancing test of the CP-Tg mice revealed better learning memory and less anxiety 16 compared with the control mice. In addition, all the heterozygous and homozygous mice shared equal phenotypes and displayed normal behavioral patterns. Altogether, these findings provide insight suggesting that up-regulated PGI 2 and down-regulated TXA 2 and PGE 2 via the transgenic approach using the COX-1-10aa-PGIS gene have notable major adverse effects in vivo. The longer lifespan of the CP Tg mice (Fig. 7) provides initial data to justify our conclusion. The observed resistance to high-fat diet-induced lipid accumulation in CP-Tg mouse liver further demonstrated the possible long-term benefits of the prevention of heart diseases by controlling the microenvironment of cellular AA metabolism in favor of PGI 2 using the COX-1-10aa-PGIS gene. An ideal transgenic approach for expression of a therapeutic gene in vivo is to maintain the ability to deactivate the gene after the desired benefit has been achieved. In our future studies, we would like to test if COX-1-10aa-PGIS activity in transgenic mice can be controlled by inhibiting PGI 2 production activity, especially by the use of COX-1 and PGIS inhibitors, such as aspirin and U-51605 20 . The availability of such options allows control of the incorporated COX-1-10aa-PGIS activity in the transgenic mice. This will be examined in our future studies.
In conclusion, the COX-1-10aa-PGIS gene composed of a single enzyme with unique triple catalytic activities has been successfully incorporated into transgenic mice, which could control the microenvironment of cellular AA metabolites to provide triple vascular protection activities by increasing the conversion of AA to PGI 2 while reducing the levels of AA available for TXA 2 and PGE 2 synthesis. The resistance to the induced thrombotic and vasoconstrictive damage caused by the incorporated COX-1-10aa-PGIS was clearly identified in vivo. Our approach represents a new vascular protective strategy because triple effects have not been successfully achieved by any drugs to date, such as aspirin or PGI 2 mimics. Thus, our findings raise the possibility that heart disease may also be treated in the future by a simple transgenic approach targeting specific organs, when ethical and safety issues have been overcome and perfected accordingly.

Materials and Methods
Animals. The CP-Tg, containing a hybrid enzyme of COX-1 linked to PGIS (COX-1-10aa-PGIS), and WT mice used in the experiments were maintained in the Animal Care Facility at the University of Houston. The animals were kept in groups of one to five mice per cage in a room with a 12-h light cycle (lights on at 6:00 AM and off at 6:00 PM) at 23 °C with food and water available ad libitum. Male and female mice were randomized across the groups, with each group having an even number of male and female mice.  subcloning procedures provided by the vector company (Invitrogen) as previously described 11,12,17,21 . The resulting cDNA was successfully subcloned into the pcDNA 3.1 vectors at Kpnl and BamHl sites containing a cytomegalovirus early promoter by PCR. The correct cDNA sequences were confirmed by DNA sequencing and restriction enzyme digestion analyses.
Construction of the cDNA plasmid to generate transgenic mice over-expressing COX-1-10aa-PGIS. The pcDNA3.1 vector containing COX-1-10aa-PGIS was cut at Nrul and Sphl sites to obtain a 3.2-kb cDNA of COX-1-10aa-PGIS with a pCMV promoter and PGH polyadenylation site (pA) as a transgene fragment. The identity of the construct was further confirmed by restriction enzyme mapping and DNA sequence analysis.
Generation of transgenic mice overexpressing COX-1-10aa-PGIS. FVB/N (Jackson Lab) female mice were maintained under a 14-hr light/10-hr dark cycle and superovulated with 5 IU of pregnant mare serum-gonadotropin followed by (after 48 hrs) 5 IU of human-chorionic gonadotropin. These females were placed with intact FVB males for mating. Fertilized oocytes were collected from the isolated oviducts of the superovulated females the following morning and treated briefly with bovine hyaluronidase in M2 medium to remove the associated debris. The COX-1-10aa-PGIS gene fragment was gel-purified using a QIAGEN kit, diluted (immediately before microinjection) to a concentration of 3 ng/μL and then microinjected into the pronuclei of fertilized oocytes using a pronuclear microinjection technique. The manipulated oocytes were transferred surgically into the oviducts of surrogate (pseudo-pregnant) recipient female mice and allowed to develop to full term to obtain the new generation of mice, which was tested for the presence of the COX-1-10aa-PGIS gene (CP-Tg). The initial procedures were performed at the University of Texas M. D. Anderson Cancer Center (Houston, TX).

Identification of the COX-1-10aa-PGIS gene in mice.
To evaluate the expression of COX-1-10aa-PGIS in the new mice, PCR analysis was performed using mouse tail tissue. Briefly, tails (1.5-2 mm) were digested in 100 μl of 1 × PCR buffer with detergents (0.45% NP40, 0.45% TWEEN 20) and 10 μl proteinase K (10 mg/ ml) at 60 °C overnight. The sample was further denatured in proteinase K by boiling for 15 min, followed by cooling on ice for 5 minutes. The isolated genomic DNA (2 µL tail DNA was added to a final reaction volume of 20 µL) was subjected to PCR analysis using PCR Reaction Buffer (1× PCR buffer, 2.5 mM MgCl 2 , 200 μM dNTPs, 1 μM each designed primer, and 1 unit Taq Polymerase under the following conditions: hold at 94 °C for 4.5 min, 30 cycles of 94 °C for 30 sec, 72 °C for 1 min, and holding at 4 °C until analysis. The primer sets used for the COX-1-10aa-PGIS gene were as follows: sense 5′-CCTCAAGGGTCTCCTAGGGA-3′ and antisense 5′-GTGCTTCTCCTTCATCCTCGT-3′. The amplified product with a length 445 bp encoded the unique region (from the COX-1 C-terminal region and the 10-aa linker to the PGIS N-terminal region) of the COX-1-10aa-PGIS hybrid enzyme. The PCR product was analyzed by agarose gel electrophoresis.
Determination of the protein expression of COX-1-10aa-PGIS in mouse tissues. The tissues were homogenized in PBS on ice and then immediately solubilized in SDS-PAGE buffer containing 2% SDS and analyzed by 7% SDS-PAGE and Western blotting as described previously 11-13,17 . Determination of the endogenous AA metabolite profiles in mice using urine samples by LC/ MS. The mouse urine was collected (n = 6) and passed through a C18 cartridge. The eluent (eluted with acetone) was dried under nitrogen gas, and the residual substrate was diluted in buffer A (containing 0.1% acetic acid and 35% acetonitrile). The prepared sample was injected into the Waters Micromass LC/MS/MS system using an auto-sampler, in which the metabolites were first separated using a RP-HPLC C18 column and then automatically injected into the mass detector equipped with an ESI source in negative mode. Synthetic AA, PGE 2 , 6-keto-PGF 1α (PGI 2 stable and final metabolite), and TXB 2 obtained from Cayman Chemical Company (Ann Arbor, MI), were used as standards to calibrate the LC/MS system, identify the corresponding prostanoids, and normalize the detection limits and sensitivities.
Bleeding time assay. The tip of the mouse tail was clipped (2 mm) with scissors, and blood was blotted onto filter paper while the time was noted at the first seconds. Thereafter, the clipped tip of the tail was blotted on a clean section of filter paper every 30 seconds until there was no longer detectable blood, at which point the total bleeding time was determined according to the following formula: Bleeding time (min) number of dots 0 5 = ×.
The bleeding time was compared between wild-type and transgenic mice.
Blood pressure and heart rate detection. The blood pressure (BP) and heart rate (HR) were measured using the tail cuff method using the CODA system from Kent Scientific Corporation, Torrington, CT. Blood pressure was measured for every individual mouse for three consecutive days to allow for acclimatization and thereby obtain more accurate measurements. Systolic, Diastolic BP, and HR were measured and plotted to compare any changes in these parameters between WT and CP-Tg mice.
Rose Bengal/Laser-induced thrombotic stroke model. The thrombotic stroke model was created by establishing photochemical vascular injury in the carotid artery of CP-Tg mice according to previously described methods [4]. Briefly, male mice were anesthetized with sodium pentobarbital (80 mg/kg, i.p.) and placed in a supine position. Then, the left common carotid artery was exposed, and a laser Doppler flow probe 407 connected to a laser Doppler Perfusion Monitor (LDPM) Unit-Periflux System (PF) 5010 was positioned on the artery to record a constant baseline blood flow. Next, the carotid artery was exposed to 1.5 mW of a green laser beam at SCiEnTifiC REPORTS | (2018) 8:1653 | DOI:10.1038/s41598-018-19661-y 540 nm (Melles Griot, CA, USA) from a distance of 5 cm and Rose Bengal (50 mg/kg) was injected through the tail vein. At this point, blood flow was constantly recorded using the accompanying software. The formation of an occlusive thrombus was indicated by the cessation of blood flow.
Determination of resistance to AA-induced thrombotic heart arrest in vivo. Sodium AA (1 mg/ ml, Sigma) in saline solution was continually infused into the mice through the tail vein. Heart beat was monitored using an ultrasound monitor (Sono Site -TITAN). The time at which the mouse heart beat stopped was used as the end-point for the AA resistance test.
Determination of angiotensin II-induced vasoconstrictive peripheral reperfusion damage. The mice were anesthetized by isoflurane inoculation. Angiotensin II (160 μg) was administered through the tail vein and peripheral blood reperfusion before and after angiotensin injections were monitored by a laser Doppler scanner (Perimed).
Determination of hepatic lipid accumulation-induced by a high-fat diet. Wild-type and transgenic mice were both fed a regular diet and a high-fat diet (Teklad, TD.01383). The diet was nutritionally complete for mice, composed of the parent 2018 diet with 2% cholesterol. The mice were fed for 6 months. After that, the mice were sacrificed, and their liver were sectioned for hematoxylin and eosin staining.