Department of Animal Science, Cornell University, Ithaca, NY 14853.
Lilly Research Laboratories, Eli Lilly and Company, Indianapolis, IN 46285.
J Dairy Sci. 2019 Dec;102(12):11586-11596. doi: 10.3168/jds.2019-16695. Epub 2019 Sep 20.
Modern dairy cows rely on hormonally driven mechanisms to coordinate the metabolic adaptations needed to meet the energy and nutrient deficits of early lactation. In the case of glucose, dairy cows cope with its scarcity during early lactation via reduced plasma concentrations of insulin and the insulin sensitizing hormone adiponectin and increased insulin resistance. Reduced insulin action promotes diversion of available glucose to the mammary gland but increases susceptibility to diseases if excessive. In earlier work, we reported that the insulin sensitizing hormone fibroblast growth factor-21 (FGF21) is increased in periparturient dairy cows and identified liver and adipose tissue as possible targets. These observations raised the possibility that FGF21 acts directly on these tissues to limit the insulin resistance of early lactation. To test this hypothesis, dairy cows were randomly assigned on d 12.6 ± 2.2 (± standard error) of lactation to receive either excipient (n = 6) or recombinant human FGF21 (n = 7), first as an FGF21 bolus of 3 mg/kg of body weight, followed 2 d later by a constant i.v. infusion of FGF21 at the rate of 6.3 mg/kg of metabolic body weight for 9 consecutive days. Biopsies of liver and adipose tissue were collected during the bolus phase of the experiment and used to analyze FGF21 signaling by Western blotting and expression of its receptor components by quantitative PCR. Bolus FGF21 administration caused a 4-fold increase in p44/42 MAPK (ERK1/2) activation in adipose tissue but had no effect on AKT and signal transducer and activator of transcription-3 (STAT3) signaling. The liver expressed negligible levels of the preferred FGF21 receptor FGFR1c and failed to mount any FGF21 signaling response. The FGF21 administered as a bolus had no effect on plasma glucose or insulin and did not stimulate an acute release of adiponectin from adipose tissue. Similarly, FGF21 infusion had no effect on plasma levels of glucose or insulin measured over the 9-d infusion or on glucose disposal during an i.v. glucose tolerance test performed on d 8 of infusion. Finally, the chronic FGF21 infusion had no effect on indices of adiponectin production, including plasma adiponectin and adipose tissue mRNA abundance of adiponectin and the endoplasmic reticulum chaperones ERO1A and DSBA-L involved in the assembly of adiponectin into multimeric complexes. These data show that human FGF21 does not act as an insulin sensitizer during the energy and glucose deficit of early lactation but do not rule out such a role in other physiological states.
现代奶牛依靠激素驱动的机制来协调代谢适应,以满足泌乳早期的能量和营养不足。就葡萄糖而言,奶牛在泌乳早期通过降低血浆胰岛素和胰岛素增敏激素脂联素的浓度以及增加胰岛素抵抗来应对其缺乏。胰岛素作用降低会促进可用葡萄糖向乳腺的转移,但如果过度则会增加患病的易感性。在早期的工作中,我们报告说,胰岛素增敏激素成纤维细胞生长因子 21(FGF21)在围产期奶牛中增加,并确定了肝脏和脂肪组织可能是靶标。这些观察结果提出了 FGF21 可能直接作用于这些组织以限制泌乳早期胰岛素抵抗的可能性。为了验证这一假设,奶牛在泌乳第 12.6 ± 2.2(±标准误差)天被随机分配接受赋形剂(n = 6)或重组人 FGF21(n = 7),首先给予 3 mg/kg 体重的 FGF21 冲击剂量,2 天后,以 6.3 mg/kg 代谢体重的恒定静脉内输注速度连续输注 FGF21 9 天。在实验的冲击阶段采集肝脏和脂肪组织活检,并用 Western blot 分析 FGF21 信号,用定量 PCR 分析其受体成分的表达。FGF21 冲击给药导致脂肪组织中 p44/42 MAPK(ERK1/2)激活增加 4 倍,但对 AKT 和信号转导和转录激活因子 3(STAT3)信号没有影响。肝脏表达的首选 FGF21 受体 FGFR1c 水平可忽略不计,并且无法产生任何 FGF21 信号反应。作为冲击给予的 FGF21 对血浆葡萄糖或胰岛素没有影响,也没有刺激脂肪组织中脂联素的急性释放。同样,在第 8 天输注期间进行静脉内葡萄糖耐量试验时,FGF21 输注对 9 天输注期间测量的血浆葡萄糖或胰岛素水平或葡萄糖处置没有影响。最后,慢性 FGF21 输注对脂联素产生的指数没有影响,包括血浆脂联素和脂肪组织中脂联素以及参与脂联素组装成多聚体复合物的内质网伴侣 ERO1A 和 DSBA-L 的 mRNA 丰度。这些数据表明,人 FGF21 在泌乳早期的能量和葡萄糖不足期间不作为胰岛素增敏剂,但不能排除其在其他生理状态下的作用。
