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DEVELOPMENTAL PHYSIOLOGY AND PREGNANCY

Inhibition of cyclooxygenase isoforms in late- but not midgestation decreases contractility of the ductus arteriosus and prevents postnatal closure in mice

¹Department of Pediatrics, Vanderbilt University, Nashville, Tennessee; and ²Cardiovascular Research Institute and Department of Pediatrics, University of California, San Francisco, San Francisco, California

Submitted 15 April 2006 ; accepted in final form 19 July 2006

	ABSTRACT

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Use of cyclooxygenase (COX) inhibitors to delay preterm birth is complicated by in utero constriction of the ductus arteriosus and delayed postnatal closure. Delayed postnatal closure has been attributed to loss of vasa vasorum flow and ductus wall ischemia resulting from constriction in utero. We used the murine ductus (which does not depend on vasa vasorum flow) to determine whether delayed postnatal closure may be because of mechanisms independent of in utero constriction. Acute inhibition of both COX isoforms constricted the fetal ductus on days 18 and 19 (term) but not earlier in gestation; COX-2 inhibition constricted the fetal ductus more than COX-1 inhibition. In contrast, mice exposed to prolonged inhibition of COX-1, COX-2, or both COX isoforms (starting on day 15, when the ductus does not respond to the inhibitors) had no contractile response to the inhibitors on days 18 or 19. Newborn mice closed their ductus within 4 h of birth. Prolonged COX inhibition on days 11–14 of gestation had no effect on newborn ductal closure; however, prolonged COX inhibition on days 15–19 resulted in delayed ductus closure despite exposure to 80% oxygen after birth. Similarly, targeted deletion of COX-2 alone, or COX-1/COX-2 together, impaired postnatal ductus closure. Nitric oxide inhibition did not prevent the delay in ductus closure. These data show that impaired postnatal ductus closure is not the result of in utero ductus constriction or upregulation of nitric oxide synthesis. They are consistent with a novel role for prostaglandins in ductus arteriosus contractile development.

patent ductus arteriosus; nonsteroidal anti-inflammatory drugs

Constriction of the ductus arteriosus can also occur in utero when NSAIDs are given to pregnant women to treat preterm labor (13, 20, 25, 30, 31, 37, 38). Surprisingly, some preterm newborn infants, who are delivered after in utero exposure to indomethacin, have an increased, rather than decreased, incidence of PDA in the newborn period; in addition, the PDA in these infants frequently fails to close with postnatal indomethacin treatment (12, 27, 34, 35). A similar finding occurs in fetal sheep that have been exposed to indomethacin for several days in utero (6, 9). The basis for this paradoxical response is not entirely clear. In the fetal sheep, indomethacin produces ductus constriction in utero, which is accompanied by cessation of ductus vasa vasorum blood flow and the development of hypoxic ischemia in the ductus muscle media. This is followed by increased production of vascular endothelial growth factor and nitric oxide and smooth muscle cell death. These in utero changes prevent the ductus from developing effective constriction after birth (6, 9). The degree of ischemia in the ductus wall is directly related to the degree of fetal ductus constriction. With advancing gestation, there is both an increase in indomethacin's ability to constrict the fetal ductus (20, 37, 38) and an increase in the thick-walled vessel's dependence on vasa vasorum flow for its oxygen delivery (14); these two observations may explain why human fetuses are more likely to have delayed postnatal ductus closure when their in utero exposure to indomethacin occurs late in gestation rather than earlier in gestation (27).

We hypothesized that prolonged in utero COX inhibition might also alter ductus contractility through mechanisms that are independent of initial ductus constriction, vasa vasorum flow, or the resultant hypoxic ischemia. In contrast to humans and sheep, the rodent ductus arteriosus has no vasa vasorum in its muscle media; the thickness of the rodent ductus is so thin that luminal blood flow is sufficient to meet all of its oxygen needs (29, 36, 40). The absence of compressible vasa vasorum in the ductus muscle media makes it less susceptible to developing hypoxia in utero during episodes of ductus constriction. In addition, although indomethacin constricts the rodent ductus arteriosus, it does so only late in gestation (23, 29). As a result, the rodent ductus is unlikely to develop hypoxic ischemia when exposed to indomethacin early in gestation. In this study, we used fetal and newborn mice after acute and chronic exposure to selective COX-1 and COX-2 inhibitors to study the nonischemic effects of prostaglandin inhibition on ductus contractility. The ductus arteriosus of mice with targeted deletions of genes encoding COX-1, COX-2, or both COX isoforms was also examined.

	MATERIALS AND METHODS

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Animals and tissues. Animals were housed in an American Association for the Accreditation of Laboratory Animal Care-approved facility and managed in accordance with National Institutes of Health animal care standards. All protocols were approved by the Vanderbilt University Institutional Animal Care and Use Committee. Wild-type female CD-1 mice (7–8 wk old; Charles River, Raleigh, NC) were bred with fertile males to produce timed pregnancies (where day 1 = presence of vaginal plug). COX-1 null (Taconic, Hudson, NY) and COX-2 null (Jackson Laboratory, Bar Harbor, ME) mice were outbred on the CD-1 background to enhance reproductive vigor (28) and facilitate comparison with wild-type CD-1 results. COX-1 and COX-2 mice on this genetic background were interbred to generate COX-1(–/–)COX-2(–/+) compound heterozygote mating pairs. Crossbreeding of COX-1(–/–)COX-2(–/+) mice was performed to generate COX-1/COX-2 double null offspring (28).

Pregnant females were anesthetized with avertin (2,2,2 tribromoethanol in tert-amyl alcohol; 0.4–0.6 mg/g body wt ip) followed by isoflurane inhalation (Baxter, Deerfield, IL) to achieve deep anesthesia and allow time for fetal anesthetic effects. Caesarian section was performed to deliver fetal pups at various gestational stages. After removal from the uterus, a transverse incision was made through the abdominal wall of anesthetized nonbreathing fetuses, and the diaphragm was opened. Skin overlying the chest wall was removed to enhance tissue fixation. Fetal tissues were preserved by immersion in chilled 4% paraformaldehyde for 24 h followed by 70% ethanol. Newborn pups were delivered by caesarean section on the morning of day 19 of pregnancy (mice in this colony typically deliver on the evening of day 19). Pups were dried and stimulated until respirations were established and then placed in prewarmed microisolator cages at 37°C for 4 h. To produce hyperoxia and accelerate ductus closure, pups were placed in FI_O2 = 0.8–1.0. At 4 h of age, newborn pups were killed by isoflurane overdose (30 s exposure), and the abdomen and diaphragm were surgically exposed. Newborn tissues were preserved in 4% paraformaldehyde followed by 70% ethanol. The thorax of preserved fetal and newborn pups was excised from surrounding tissues and embedded in paraffin. The thorax was sectioned in a plane parallel to the diaphragm. Ribbons of serial 6-µm sections containing heart and outflow tracts were mounted on poly-L-lysine-coated slides and stained with hematoxylin.

Drug administration. COX inhibitors were administered at different time points during mid- and late gestation according to treatment protocol (Fig. 1). All drugs have been previously shown to cross the placenta (17). Selective COX inhibitors were reconstituted in a 0.1% methylcellulose solution and continuously stirred before administration. Caesarian deliveries were performed at noon, 4 h after the final dose of any drug was administered. Protocols A-D addressed the fetal ductus arteriosus, whereas protocols E-G addressed the newborn ductus arteriosus. In protocol A, pregnant wild-type females received either a single dose of indomethacin (5.0 mg·kg^–1·dose^–1 ip; Merck, West Point, PA), a selective inhibitor of COX-1 (SC560, 30 mg·kg^–1·dose^–1, 0.2 ml gavage), or a selective COX-2 inhibitor (SC236, 15 mg·kg^–1·dose^–1; 0.2 ml gavage; Cayman Chemical, Ann Arbor, MI) at 0800 on day 19 of gestation. Fetal tissues were harvested 4 after the last drug dosage. In protocol B, pregnant females were chronically treated with either SC560 (30 mg·kg^–1·dose^–1 two times daily; 0.2 ml gavage), SC236 (15 mg·kg^–1·dose^–1 every other day; 0.2 ml gavage), or both compounds from day 15–19 of gestation (term = day 19). Fetal tissues were harvested 4 h after the last drug dosage. In some experiments, COX-1 null females were treated with SC236 on days 15–19 of gestation according to the schedule in protocol B. Because of signs of dehydration and lethargy in COX-1 null females treated with the COX-2 inhibitor, omeprazole (100 mg·kg^–1·dose^–1; Calbiochem, San Diego, CA) was given by gavage one time daily. In protocol C, pregnant wild-type females were treated with a single dose of both SC560 and SC236 at 0800 on either day 16, 17, 18, or 19 of gestation; fetal tissues were harvested 4 h after the drug dosage on each respective day. In protocol D, pregnant wild-type females were chronically treated with both SC560 and SC236 on days 15–18 of gestation. Fetal tissues were harvested 4 h after the final drug dosage on day 18. In protocol E, pregnant wild-type females were chronically treated with both SC560 and SC236 on days 11–14 of gestation. Pregnancy was allowed to continue until caesarian section at term gestation. Tissues were harvested from newborn pups after 4 h of oxygen exposure. In protocol F, pregnant females were chronically treated with either SC560, SC236, or both compounds from day 15–19 of gestation (similar to protocol B). Newborn tissues were harvested after 4 h of postnatal oxygen exposure. In protocol G, pregnant females were chronically treated with both SC560 and SC236 from day 15–19 of gestation (same drug dosage as protocol B). Newborn litters were divided into thirds, and pups were treated with one of the following: the nonselective nitric oxide synthase (NOS) inhibitor N^G-nitro-L-arginine methyl ester (L-NAME, 100 mg·kg^–1·dose^–1; Cayman Chemical), the thromboxane receptor agonist U-46619 (0.5 µg/mouse; Cayman Chemical) given at birth and 1.5 and 3 h of age, or 10 µl sterile saline. Compounds were injected through the nuchal fold to form a subcutaneous pocket along the back under direct visualization by stereomicroscopy. Pups with leaking injection sites were excluded from analysis.

View larger version (18K): [in this window] [in a new window]   Fig. 1. Drug treatment protocols. Pregnant dams were treated with a nonselective cyclooxygenase (COX) inhibitor [indomethacin (Indo)], a selective COX-1 inhibitor (SC560), and/or a selective COX-2 inhibitor (SC236) on the indicated days of gestation [day (d) 1 = presence of vaginal plug]. Fetal studies: protocol A examined the effects of a single dose of a COX inhibitor (either indomethacin, SC236, SC560, or the combination of SC236 with SC560) on the fetal ductus (tissue collected 4 h after treatment); protocol B examined the effects of prolonged COX-1, COX-2, or combined COX-1 and COX-2 inhibition on the fetal ductus (study drugs were administered at the indicated times, and the tissues were harvested 4 h after the last dose); protocol C examined the effects of a single treatment with both COX-1 and COX-2 inhibitors on the fetal ductus. Pregnant dams were treated at either gestation day 16, 17, 18, or 19, and the fetal tissues were harvested 4 h later; protocol D examined the effects of prolonged COX-1 and COX-2 inhibition on the fetal ductus at day 18 of gestation. Pregnant dams were treated on days 15–18 of gestation, and the fetal tissues were harvested 4 h after the last dose on day 18. Newborn studies: protocol E examined the effects of prolonged COX-1 and COX-2 inhibition (on days 11–14 of gestation) on the newborn ductus. Newborn tissues were harvested 4 h after delivery; protocol F examined the effects of prolonged in utero exposure to either COX-1, COX-2, or combined COX-1 and COX-2 inhibitors (on days 15–19 of gestation) on the newborn ductus. Newborn tissues were harvested 4 h after delivery; protocol G examined whether treatment of newborn littermates with NG-nitro-L-arginine methyl ester (L-NAME) or U-46619 (or saline) altered patency of the ductus arteriosus (after prolonged in utero exposure to both COX inhibitors on days 15–19 of gestation). PP1, postpartum day 1.

View larger version (153K): [in this window] [in a new window]   Fig. 2. Physiological closure of the mouse ductus arteriosus. Anatomical views of the open fetal ductus arteriosus on the morning of day 19 of gestation (A) and constricted newborn ductus arteriosus at 4 h of age (B). Serial thoracic sections demonstrate histologic features and dimensions of the open fetal ductus (C) and adjacent transverse aortic arch (E) compared with the closed newborn ductus (D) and corresponding transverse aortic arch (F). aAO, ascending aorta; tAO, transverse aorta; dAO, descending aorta; PA, pulmonary artery; DA, ductus arteriosus; Tra, trachea; Eso, esophagus, VB, vertebral body.

	RESULTS

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View larger version (13K): [in this window] [in a new window]   Fig. 3. Response of the fetal ductus arteriosus to acute and chronic COX-1 or COX-2 inhibition. Fetuses of wild-type dams treated with indomethacin, a selective COX-1 inhibitor (SC560), or selective COX-2 inhibitor (SC236) were compared. Vessel dimensions are expressed as a ratio of ductus arteriosus (DA) and transverse aorta (AO) diameters. A: acute pharmacological inhibition with indomethacin (n = 6, 2 litters) or combined COX inhibitors (n = 19, 7 litters) showed similar ductus constriction at term gestation compared with untreated (No Tx) controls (n = 11, 6 litters). Acute COX-1 inhibition (n = 9, 3 litters) caused less ductus constriction than COX-2 (n = 11, 4 litters). B: chronic COX-1 (n = 9, 3 litters), COX-2 (n = 35, 12 litters), or combined COX inhibition (n = 20, 6 litters) did not constrict the fetal ductus. P < 0.05 compared with control (*) and compared with SC560 ().

View larger version (15K): [in this window] [in a new window]   Fig. 4. Developmental stage-specific response of the fetal ductus arteriosus to acute and chronic COX inhibition. Fetuses of wild-type dams treated with combined COX-1 (SC560) and COX-2 (SC236) inhibitors were compared. Vessel dimensions are expressed as a ratio of DA and AO diameters. A: acute inhibition of both COX isoforms did not alter the day 16 (n = 9, 3 litters) or day 17 (n = 9, 3 litters) gestation ductus but induced constriction on day 18 (n = 13, 4 litters) and day 19 (n = 19, 7 litters). B: in contrast to the acute responses, chronic exposure to both COX inhibitors, starting on day 15, was not associated with ductus constriction on either day 18 (n = 12, 3 litters) or day 19 (n = 20, 6 litters). *P < 0.05 compared with vehicle-treated dams at each gestation.

Failure of newborn ductus arteriosus closure after exposure to chronic COX inhibition in utero. We examined the effects of chronic in utero COX inhibition on the ability of the newborn ductus to constrict after birth. Newborns were delivered by caesarean section and exposed to 80% oxygen for 4 h. Control pups, born to dams that did not receive COX inhibitors during pregnancy, closed their ductus completely by 4 h after delivery (Fig. 5A, compare with fetal dimensions in Fig. 2B). Newborn pups, born to dams that received both COX-1 and COX-2 inhibitors in midpregnancy, on days 11–14 of gestation (protocol E) also had complete ductus closure by 4 h after delivery. In contrast, newborn pups exposed to both COX inhibitors on days 15–19 of gestation (protocol F) had incomplete constriction of their ductus (Fig. 5A). There was no significant difference between the treated (SC560 + SC236) and control groups in mixed arterial-venous blood PO₂ samples obtained by cervical transection after 4 h of postnatal oxygen exposure (PO₂: 101.5 ± 28, n = 5 vs. 89.1 ± 14, n = 8, respectively). Prolonged exposure to either COX-1 or COX-2 inhibitor alone also resulted in incomplete closure of the newborn ductus (Fig. 5A).

View larger version (16K): [in this window] [in a new window]   Fig. 5. Ductus contractility in the newborn mouse after genetic and/or prolonged pharmacological COX inhibition in utero. A: newborn pups born to dams with chronic COX-1 (SC560), COX-2 (SC236), or combined COX inhibitors were placed in 80% oxygen for 4 h after birth. Vessel dimensions are expressed as a ratio of DA and AO diameters. Chronic COX inhibition on days 11–14 of gestation (n = 20, 7 litters) did not alter ductus closure after birth, whereas pups with COX-1 (n = 12, 4 litters), COX-2 (n = 23, 13 litters), or combined COX inhibition (n = 29, 11 litters) on days 15–19 of gestation had delayed closure of the ductus compared with controls (n = 12, 4 litters). B: targeted deletion of COX-1 (n = 11, 4 litters) had minimal effect on ductus closure after birth, whereas COX-2 deletion (n = 20, 8 litters) and COX-1/COX-2 double-null pups (n = 12, 6 litters) had a significant delay in ductal closure compared with controls (n = 12, 4 litters). Closure of the ductus of COX-1 null pups chronically exposed to COX-2 inhibitor in utero (n = 16, 6 litters) was also significantly delayed. KO, knockout. *P < 0.05 compared with untreated newborns at 4 h of age.

Impaired response of newborn PDAs to vasoconstrictive stimuli. We examined whether the persistent postnatal PDA that follows chronic in utero COX inhibition might be due, in part, to increased nitric oxide production (3). Fetuses that were exposed to both COX-1 plus COX-2 inhibitors in utero (on days 15–19 of gestation) were delivered by caesarean section and either treated with saline or the nonspecific NOS inhibitor L-NAME (protocol G). The L-NAME-treated newborns had the same degree of ductus patency as the saline-treated controls (Fig. 6). The effect of NOS inhibition was also examined in COX-1 null mice that were chronically treated with COX-2 inhibitors on days 15–19 of gestation. Newborns from these dams showed no difference in ductus caliber between saline-treated pups and pups that were treated with L-NAME (Fig. 6).

View larger version (17K): [in this window] [in a new window]   Fig. 6. Responsiveness of the newborn patent ductus arteriosus. Newborn pups born to dams with chronic COX-1 (SC560) plus COX-2 (SC236) inhibition on days 15–19 of gestation were placed in 80% oxygen for 4 h after birth. Vessel dimensions are expressed as a ratio of DA and AO diameters. Ductus closure rates of pups treated with saline (n = 24, 12 litters), L-NAME (n = 21, 6 litters), or U-46619 (n = 24, 7 litters) were significantly delayed compared with untreated controls (n = 12, 4 litters; P < 0.05) but did not differ between the treatment groups. Similarly, there was no difference in ductus caliber between saline-treated (n = 15, 5 litters) and L-NAME-treated (n = 14, 4 litters) COX-1 null pups chronically exposed to COX-2 inhibitor in utero.

	DISCUSSION

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We found that inhibition of prostaglandin production has different effects on ductus patency depending on developmental stage and duration of treatment. Acute inhibition of either COX isoform led to fetal ductus constriction, with the inhibition of COX-2 having greater effects than those of COX-1. The constrictive effects of acute COX inhibition were not apparent until day 18 of gestation (last 10% of gestation). Our findings are consistent with previous studies in mice (29), rats (22), and humans (20, 37, 38).

In contrast, prolonged COX inhibition during the last 25% of gestation did not induce fetal ductus constriction; rather, it led to impaired contractile responses in the near-term fetus and a persistent PDA in the newborn mouse. Combined COX gene deletion had similar effects in delaying ductus closure as prolonged pharmacological COX inhibition. This finding is similar to previous reports (17). In contrast to the ovine ductus (6, 9), the inhibitory effects of prolonged COX inhibition in the full-term mouse did not appear to be because of prior vasa vasorum hypoperfusion secondary to in utero ductus constriction. First, the muscle media of the fetal mouse ductus has no vasa vasorum (29, 36, 40), and, second, no change in ductus diameter was observed throughout gestation (Fig. 4) since the prolonged COX inhibition was started at a time when COX inhibition does not contract the fetal ductus (day 15, see Fig. 4). One possible explanation for the delayed closure after prolonged COX inhibition is that prolonged COX inhibition results in the upregulation of other vasodilators. Functional coupling of COX and NOS systems is a well-recognized phenomenon (10, 18, 21). In the mouse ductus arteriosus, endothelial NOS is the predominant isoform for nitric oxide production, and its expression is stable in mid- to late gestation (29). Baragatti et al. (3) recently hypothesized that absence of COX-derived prostaglandins in utero may lead to an increase in nitric oxide production in the ductus; they found that the NOS inhibitor L-NAME produced a stronger contractile response in isolated ductus from COX-1 null or COX-2 null fetal mice than from wild-type mice. Although functional coupling of COX and NOS systems may occur locally within the ductus, it does not appear to explain the decreased contractility of the postnatal ductus after prolonged COX inhibition in vivo; we observed no increase in postnatal ductus constriction when fetuses that were chronically exposed to COX inhibition in utero were treated with L-NAME after birth (Fig. 6).

Our studies suggest that prostaglandins may have a unique and previously unappreciated role in the development of pathways that control ductus contractility to any vasoactive stimulus. For example, after chronic in utero COX inhibition, the thromboxane mimetic U-46619 has no effect on the degree of ductus patency even when used at doses that previously have been shown to constrict the neonatal ductus (Fig. 6 and Refs. 17 and 33). Muscular development of the ductus is marked by precocious differentiation of specific myosin isoforms (15) and cytoskeletal proteins (4, 8, 32) that appear to play a role in its postnatal closure and remodeling. Interruption of smooth muscle differentiation leads to delayed postnatal ductus closure (24). Prostaglandins play an important role in vascular smooth muscle migration and differentiation (1, 16, 19). We hypothesize that prolonged COX inhibition on days 15–19 of gestation alters the development of the contractile apparatus that is essential for rapid constriction after birth. Our results also suggest that days 15–19 of gestation span the critical period of contractile development since ductus contractility was unaffected when mice were exposed to combined COX inhibition at an earlier time in gestation (days 11–15 of gestation; Fig. 5).

Although both COX-1 and COX-2 affect the development of ductus contractility, they do so to different degrees. Our results are similar to the observations of Loftin et al. (17) where chronic COX-2 inhibition on days 16–19 of gestation resulted in a postnatal PDA, whereas chronic COX-1 inhibition over the same period did not. We observed a small but significant PDA after chronic COX-1 inhibition on days 15–19 of pregnancy (Fig. 5). This discrepancy may be explained by a longer duration of COX-1 inhibition in our studies, strain differences in susceptibility to COX inhibition, or different environmental conditions that alter COX functions (2, 39). Nevertheless, our data clearly show that prolonged inhibition of either COX-1 or COX-2 alone impairs ductal constriction after birth and is not the result of in utero constriction of the fetal ductus. Mice with targeted deletion of the PGE₂ receptor EP₄ have a similar PDA phenotype (26), suggesting that a specific prostaglandin receptor pathway may regulate the development of ductus arteriosus contractility.

In summary, we suggest that prostaglandins may play a novel role in ductus arteriosus development that is distinct from their function as a mediator of vascular tone. A better understanding of this process will be important for the development of new strategies to treat preterm labor without affecting fetal vascular development.

	GRANTS

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This work was supported by National Institutes of Health Grants HL-77395 (to J. Reese), HL-46691, and HL-56061 (to R. I. Clyman), American Heart Association Grant AHA455360 (to J. Reese), and by gifts from the Philip S. Astrowe Trust (to J. Reese) and the B and J Gates Foundation (to R. I. Clyman).

	FOOTNOTES

 

Address for reprint requests and other correspondence: J. Reese, 1125 MRB IV Bldg., 2215 B Garland Ave, Dept. of Pediatrics, Vanderbilt Univ. Medical Center, Nashville, TN 37232-0656 (e-mail: jeff.reese{at}vanderbilt.edu)

The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

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