2006
DOI: 10.1159/000088842
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β<sub>1</sub>-Adrenergic Receptors Maintain Fetal Heart Rate and Survival

Abstract: β-Adrenergic receptor (βAR) activation has been shown to maintain heart rate during hypoxia and to rescue the fetus from the fetal lethality that occurs in the absence of norepinephrine. This study examines whether the same subtype of βAR is responsible for survival and heart rate regulation. It also investigates which βARs are located on the early fetal heart and whether they can be directly activated during hypoxia. Cultured E12.5 mouse fetuses were treated with subtype-specific βAR antagonists to pharmacolo… Show more

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Cited by 16 publications
(20 citation statements)
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“…In the early fetus, hypoxia slows heart rate to a greater extent in catecholamine-deficient fetuses than in wild-type (wt) siblings. This reduction is completely reversed by ␤-AR agonists (6,41), consistent with the view that released NE increases heart rate during hypoxia in wt animals. Because cardiac output in the fetus is primarily dependent on heart rate (reviewed in Ref.…”
supporting
confidence: 88%
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“…In the early fetus, hypoxia slows heart rate to a greater extent in catecholamine-deficient fetuses than in wild-type (wt) siblings. This reduction is completely reversed by ␤-AR agonists (6,41), consistent with the view that released NE increases heart rate during hypoxia in wt animals. Because cardiac output in the fetus is primarily dependent on heart rate (reviewed in Ref.…”
supporting
confidence: 88%
“…Hypoxic wt fetuses are bradycardic (6,41) and show signs of congestive heart failure, myocardial thinning, and epicardial detachment (44).…”
Section: Thmentioning
confidence: 99%
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“…RNA samples were reverse transcribed in the presence of 5X First strand buffer, 10 mmol/ L DTT, random hexamer primers, and SuperScript RTIII. Complementary DNA (cDNA) synthesis was carried out in a thermocycler at 25 C/10 min, 42 C/50 min, 72 C/10 min, and 4 C. Real time reverse transcriptionÀpolymerase chain reaction (RT-PCR) assay was then performed by the DDCt method 17 using the TaqMan probe set for human b 1 -AR (Hs00265096_s1; Applied Biosystems, California) and b 2 -AR (Hs00240532_s1; Applied Biosystems) on an ABI 7900 Sequence Detection System. In each experiment, mRNA levels were normalized to 18S ribosomal RNA (rRNA; measured using TaqMan Gene Expression Assay for 18S, #Hs99999901_s1, from Applied Biosystems), which did not change under experimental conditions (data not shown).…”
Section: Quantitative Reverse Transcriptionàpolymerase Chain Reactionmentioning
confidence: 99%