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Fig. 6. Contribution of the H2S precursor, cysteine, to hypoxic
responses. (A) Addition of cysteine to lamprey dorsal aorta (DA) significantly
and specifically increases the magnitude of a hypoxic contraction. In the
absence of exogenous cysteine, a hypoxic contraction (N2) develops
as much force as a reference 80 mmol l–1 KCl contraction
(broken line). Addition of cysteine (Cys; 1 mmol l–1)
produces a slight, transient contraction, doubles the strength of the hypoxic
contraction (N2+Cys; P
0.05), but does not affect a
second KCl contraction. Addition of glycine (Gly; 1 mmol l–1)
also produced a slight contraction but did not affect either hypoxic
(N2+GLY) or KCl (KCl+Gly) contractions. (B) Rat thoracic aortas
(TA) were exposed to hypoxia for 15 h in the absence (Con) or presence of
cysteine (Cys), returned to normoxia, pre-contracted with U-46619, and exposed
twice to hypoxia. Incubation with cysteine significantly (P0.05)
reduced the magnitude of the first hypoxic relaxation but enabled the vessels
to respond to re-oxygenation and a second hypoxia. (C) Bovine pulmonary
arteries (PA) were exposed to hypoxia for 15 h in the absence (Con) or
presence of cysteine (Cys), returned to normoxia, pre-contracted with U-46619,
and exposed twice to hypoxia. Incubation with cysteine increased the magnitude
of the initial hypoxic contraction and the second hypoxic contraction was
sustained longer.
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