Mukhopadhyay S, Cowsik S M, Lynn A M, Welsh W J, Howlett A C
Department of Pharmacological and Physiological Science, Saint Louis University School of Medicine, Missouri 63104, USA.
Biochemistry. 1999 Mar 16;38(11):3447-55. doi: 10.1021/bi981767v.
A CB1 cannabinoid receptor peptide fragment from the C-terminal juxtamembrane region autonomously inhibits adenylyl cyclase activity in a neuroblastoma membrane preparation. The cannabinoid receptor antagonist, SR141716A, failed to block the response. The peptide was able to evoke the response in membranes from Chinese hamster ovary (CHO) cells that do not express the CB1 receptor. These studies are consistent with a direct activation of Gi by the peptide. To test the importance of a BXBXXB sequence, Lys403 was acetylated, resulting in a peptide having similar affinity but reduced efficacy. N-Terminal truncation of Arg401 resulted in a 6-fold loss of affinity, which was not further reduced by sequential truncation of up to the first seven amino acids, four of which are charged. N-Terminal-truncated peptides exhibited maximal activity, suggesting that Gi activation can be conferred by the remaining amino acids. Truncation of the C-terminal Glu417 or substitution of Glu417 by a Leu or of Arg401 by a Norleucine reduced activity at 100 microM. The C-terminal juxtamembrane peptide was constrained to a loop peptide by placement of Cys residues at both terminals and disulfide coupling. This modification reduced the affinity 3-fold but yielded near-maximal efficacy. Blocking the Cys termini resulted in a loss of efficacy. Circular dichroism spectropolarimetry revealed that all C-terminal juxtamembrane peptide analogues exist in a random coil conformation in an aqueous environment. A hydrophobic environment (trifluoroethanol) failed to induce alpha-helix formation in the C-terminal juxtamembrane peptide but did so in less active peptides. The anionic detergent sodium dodecyl sulfate induced alpha-helix formation in all analogues except the loop peptide, where it induces a left-handed PII conformation. It is concluded that alpha-helix formation is not required for Gi activation.
来自C末端近膜区的CB1大麻素受体肽片段在神经母细胞瘤膜制剂中可自主抑制腺苷酸环化酶活性。大麻素受体拮抗剂SR141716A未能阻断该反应。该肽能够在不表达CB1受体的中国仓鼠卵巢(CHO)细胞的膜中引发反应。这些研究与该肽直接激活Gi一致。为了测试BXBXXB序列的重要性,将Lys403乙酰化,得到一种具有相似亲和力但效力降低的肽。Arg401的N末端截短导致亲和力丧失6倍,进一步截短至前七个氨基酸(其中四个带电荷)并没有进一步降低亲和力。N末端截短的肽表现出最大活性,表明剩余的氨基酸可以赋予Gi激活能力。C末端Glu417的截短或用Leu取代Glu417或用正亮氨酸取代Arg401在100μM时降低了活性。通过在两个末端放置半胱氨酸残基并进行二硫键偶联,将C末端近膜肽限制为环肽。这种修饰使亲和力降低了3倍,但产生了接近最大的效力。封闭半胱氨酸末端导致效力丧失。圆二色光谱偏振法显示,所有C末端近膜肽类似物在水性环境中均以无规卷曲构象存在。疏水环境(三氟乙醇)未能在C末端近膜肽中诱导α螺旋形成,但在活性较低的肽中能诱导形成。阴离子去污剂十二烷基硫酸钠在除环肽外的所有类似物中诱导α螺旋形成,在环肽中诱导左手PII构象。结论是,Gi激活不需要α螺旋形成。
