Delgado Yamixa, Morales-Cruz Moraima, Hernández-Román José, Martínez Yashira, Griebenow Kai
Department of Biology, University of Puerto Rico, Río Piedras Campus, P,O, Box 70377, San Juan, Puerto Rico 00931-3346, USA.
BMC Biochem. 2014 Aug 6;15:16. doi: 10.1186/1471-2091-15-16.
Cytochrome c (Cyt c) is an apoptosis-initiating protein when released into the cytoplasm of eukaryotic cells and therefore a possible cancer drug candidate. Although proteins have been increasingly important as pharmaceutical agents, their chemical and physical instability during production, storage, and delivery remains a problem. Chemical glycosylation has been devised as a method to increase protein stability and thus enhance their long-lasting bioavailability.
Three different molecular weight glycans (lactose and two dextrans with 1 kD and 10 kD) were chemically coupled to surface exposed Cyt c lysine (Lys) residues using succinimidyl chemistry via amide bonds. Five neo-glycoconjugates were synthesized, Lac4-Cyt-c, Lac9-Cyt-c, Dex5(10kD)-Cyt-c, Dex8(10kD)-Cyt-c, and Dex3(1kD)-Cyt-c. Subsequently, we investigated glycoconjugate structure, activity, and stability. Circular dichroism (CD) spectra demonstrated that Cyt c glycosylation did not cause significant changes to the secondary structure, while high glycosylation levels caused some minor tertiary structure perturbations. Functionality of the Cyt c glycoconjugates was determined by performing cell-free caspase 3 and caspase 9 induction assays and by measuring the peroxidase-like pseudo enzyme activity. The glycoconjugates showed ≥94% residual enzyme activity and 86 ± 3 to 95 ± 1% relative caspase 3 activation compared to non-modified Cyt c. Caspase 9 activation by the glycoconjugates was with 92 ± 7% to 96 ± 4% within the error the same as the caspase 3 activation. There were no major changes in Cyt c activity upon glycosylation. Incubation of Dex3(1 kD)-Cyt c with mercaptoethanol caused significant loss in the tertiary structure and a drop in caspase 3 and 9 activation to only 24 ± 8% and 26 ± 6%, respectively. This demonstrates that tertiary structure intactness of Cyt c was essential for apoptosis induction. Furthermore, glycosylation protected Cyt c from detrimental effects by some stresses (i.e., elevated temperature and humidity) and from proteolytic degradation. In addition, non-modified Cyt c was more susceptible to denaturation by a water-organic solvent interface than its glycoconjugates, important for the formulation in polymers.
The results demonstrate that chemical glycosylation is a potentially valuable method to increase Cyt c stability during formulation and storage and potentially during its application after administration.
细胞色素c(Cyt c)释放到真核细胞胞质中时是一种引发凋亡的蛋白质,因此是一种潜在的抗癌药物候选物。尽管蛋白质作为药物制剂越来越重要,但其在生产、储存和递送过程中的化学和物理不稳定性仍然是一个问题。化学糖基化已被设计为一种增加蛋白质稳定性从而提高其长效生物利用度的方法。
使用琥珀酰亚胺化学通过酰胺键将三种不同分子量的聚糖(乳糖以及两种分子量分别为1 kD和10 kD的葡聚糖)化学偶联到表面暴露的Cyt c赖氨酸(Lys)残基上。合成了五种新的糖缀合物,即Lac4-Cyt-c、Lac9-Cyt-c、Dex5(10kD)-Cyt-c、Dex8(10kD)-Cyt-c和Dex3(1kD)-Cyt-c。随后,我们研究了糖缀合物的结构、活性和稳定性。圆二色性(CD)光谱表明,Cyt c糖基化不会导致二级结构发生显著变化,而高糖基化水平会引起一些轻微的三级结构扰动。通过进行无细胞半胱天冬酶3和半胱天冬酶9诱导试验以及测量过氧化物酶样假酶活性来确定Cyt c糖缀合物的功能。与未修饰的Cyt c相比,糖缀合物显示出≥94%的残余酶活性以及86±3%至95±1%的相对半胱天冬酶3激活率。糖缀合物对半胱天冬酶9的激活率在误差范围内为92±7%至96±4%,与半胱天冬酶3的激活率相同。糖基化后Cyt c的活性没有重大变化。用巯基乙醇孵育Dex3(1 kD)-Cyt c会导致三级结构显著丧失,半胱天冬酶3和9的激活率分别降至仅24±8%和26±6%。这表明Cyt c的三级结构完整性对于凋亡诱导至关重要。此外,糖基化可保护Cyt c免受某些应激(即高温和高湿度)的有害影响以及蛋白水解降解。此外,未修饰的Cyt c比其糖缀合物更容易在水-有机溶剂界面发生变性,这对于聚合物制剂很重要。
结果表明,化学糖基化是一种在制剂和储存期间以及给药后应用过程中增加Cyt c稳定性的潜在有价值的方法。
Zotero 插件
