Clinical significance of serum biochemistry changes in mice with targeted disruption of βB2-crystallin gene

AIM: To explore the pathogenesis, influencing factors, ways of medical intervention and evaluation indicators of cataract by observing changes in serum biochemical indices in mice with targeted disruption of βB2-crystallin. · METHODS: Nine 6-week-old male mice with targeted knockout of βB2-crystallin were used as the study group, and nine age- and sex-matched normal wild-type mice as the control group. The genetype of the modeled mice was identified by PCR technique. Tropicamide and phenylephrine eye drops were used as the cycloplegic agents to observe changes in lens opacity with a slit-lamp. The lens was then removed and blood was collected for biochemical evaluation in the serum. · RESULTS: Two genotypes were successfully identified by PCR technique. Slit-lamp observation showed that the lens cortex was opaque and GSH level in the lens cortex was remarkably decreased in mice with βB2-crystallin deficiency compared with the control group (P <0.01). Serum Na+, Cl-, Ca2+, Mg2+ and Fe2+ levels, ALT and AST activities, and TP, ALP, Cr, TC, GLU content were decreased significantly compared with the control group (P <0.05). There was no difference in LDH, P, Cu2+, K+ levels between the two groups (P >0.05). · CONCLUSION: Compared with the wild-type mice, serum biochemical indices underwent significant changes in mice with targeted disruption of βB2-crystallin gene, especially with abnormal distribution of Na+&Ca2+, which induced the formation of cataract.

STUDIES ON THE PORE FORMATION MECHANISM OF β-CRYSTALLINE POLYPROPYLENE UNDER STRETCHING

The pore formation mechanism of β-crystalline polypropylene under stretching was investigated. The porosity of the samples increases rapidly with stretching, having a maximum at draw ratios around 2 and then decreases monotonically. An abrupt formation process of initial micropores at very low draw ratios was evidenced by in situ SAXS measurements. At the same time the phase transition from β-crystal to α-crystal proceeds slowly in the whole deformation process up to large draw ratios around 5. Comparative studies of α-and β-crystalline polypropylene samples before stretching indicate that in addition to difference in crystal forms the α-and β-crystalline polypropylene samples exhibit quite different morphological features. There are a lot of interfaces in β-crystalline polypropylene samples, which may have a lower density value and can be easily etched by argon ions and penetrated by small molecules. It was concluded from these experimental facts that the pore formation and crystal transition are two independent phenomena during the deformation of β-crystalline polypropylene samples, and phase transition from β-crystal to α-crystal could hardly be the origin of pore formation. A defect initiation mechanism was proposed to understand the pore formation behavior of β-crystalline polypropylenes.

MULTIPLE MELTING BEHAVIOR OF β-CRYSTALLINE PHASE POLYPROPYLENE

Differential scanning calorimetry and X-ray diffraction experiments on β-nucleated polypropylene were made on the samples crystallized at different temperatures and processed by injection molding. The crystal perfection was shown to vary with crystallization temperature. The observed multiple peaks could be related to a ill-phase with defective inclination of the chains, a recrystallized or original β_2-phase of more perfect inclination, and the α-phase. Injection molded samples could be analyzed from the established DSC interpretation.

Thermal-induced Unfolding of β-Crystallin and Disassembly of its Oligomers Revealed by Temperature-Jump Time-Resolved Infrared Spectroscopy

β-Crystallins are the major structural proteins existing in the vertebrate lens, and their conformational stability is critical in maintaining the life-long transparency and refraction index of the lens. Seven subunits of β-crystallins naturally assemble into various heteroge- neous oligomers with different sizes. Here, we systematically investigated the thermal sta- bility of the different secondary structures present in β-Crystallins and then the dynamic process for the thermal-induced unfolding of β-crystallins by Fourier transform infrared spectroscopy-monitored thermal titration and temperature-jump nanosecond time-resolved IR difference absorbance spectra. Our results show that the N-terminal anti-parallel β-sheets in β-crystallin are the most unstable with a transition midpoint temperature at 36.0-2.1℃, leading to the formation of an intermediate consisting vastly of random coil structures. This intermediate structure is temporally assigned to that of the monomer generated by the thermal-induced disassembly of β-crystallin oligomers with a transition midpoint tempera- ture of 40.4-0.7℃. The global unfolding of β-crystallins that leads to denaturation and aggregation indicated by the formation of intermolecular anti-parallel β-sheets has a transi- tion midpoint temperature determined as 72.4-0.2 ℃. Temperature-jump time-resolved IR absorbance difference spectroscopy analysis further reveals that thermal-induced unfolding of β-crystallins occurs firstly in the anti-parallel β-sheets in the N-terminal domains with a time constant of 50 ns.

Structure and interactions in α-crystallin probed through thiol group reactivity

a-Crystallin is the major structural protein of eye lens of vertebrates. In human lens, the ratio of aA-crystallin to aB-crystallin was found to be 3:1. aA-Crystallin contains two cysteine residues at positions 131 and 142, which are at the junction between the a-crystallin domain and the C-terminal tail. We used the accessibility of the thiol groups by Ellman’s reagent (DTNB) as a tool to gain information about the various structural perturbations of hinge region of a-crystallin and during the binding with substrates. In the native condition, the cys-142 though reacted quite fast was not fully exposed. Several reagents were used to see the accessibility of cys-131. Rate constant for cys-131 was increased gradually with increase in the concentration of reagents. The bindings of substrates are affected by the accessibility of thiol indicating that the substrates bind to the hinge region of a-crystallin. By blocking of cys-142, it was observed that the accessibility of one thiol depends on the other thiol, and they are not independent. The hinge region of a-crystallin is very important as substrate binding site and from this study we have got various structural information about that region.

Comparative Studies of the Carbohydrate of Human Gamma-Crystallins from Fetal and Adult Lenses with Agglutinins

Using gel chromatography of Sephadex G-75 superfine connectedwith Sephadex G-50 fine column,three human γ- crystallins(γ1,γ2,γ3)couldbe obtained.Seven agglutinins(LCA,SBA,DBA,PNA,BSL,RCA and UEA)were used to detect the sugar of sub-γ-crystallins,which had been transferredto nitrocellulose membrane and finally stained with ABC reagents and the sub-strate of HPR.These results suggested that γ2-and γ3-crystallin contain sugar,but γ1-crystallin has no sugar.There is a decrease of carbohydrate of γ2 and γ3as...

Potassium Iodide and Acrylamide Fluorescence Quenching Studies on Gamma-Crystallins of Human Lenses in Development and Aging

γ_1-γ_2-and γ_3-crystallin(corresponding to γs-,γC-and γD- crys-tallin respectively)of human fetal,2 year and 20^+ year old lenses areseparated by Sephadex gel chromatography.lodide and acrylamide are usedto quench the tryptophane fluorescence of sub-γ-crystalline fractions and Ksvand fa values are calculated.The results show that iodide has no clear quench-ing effects on all γ-crystallins,the quenching effects of acrylamide on the tryp-tophan fluorescences of γ1-γ2-and γ3-crystallin from lenses of the ...

视网膜α-crystallins在增生性视网膜疾病中的研究进展

α-crystallins是小分子热休克蛋白家族(small-molecule heat shock protein,sHSP)的重要成员,包括αA-crystallin和αB-crystallin,在各类组织细胞中具有细胞保护和分子伴侣功能。近年来,多项研究发现,视网膜组织α-crystallins可利用自身特性通过各种途径参与增生性视网膜病的血管新生、上皮/内皮细胞间质化等过程。本文主要介绍α-crystallins,尤其是αB-crystallin调节增生性视网膜疾病发展的分子机制,探讨其潜在的临床应用价值。

αB-晶状体蛋白在先天性白内障大鼠晶状体中免疫活性的变化

目的观察正常以及先天性白内障大鼠晶状体中αB-晶状体蛋白的免疫活性变化,探讨其与白内障发病的关系。方法分别摘取8周龄、10周龄、12周龄、14周龄正常对照组以及先天性白内障大鼠晶状体,应用抗生物素蛋白-生物素-过氧化物酶复合体法,观察不同时期大鼠晶状体中αB-晶状体蛋白的免疫活性变化。结果αB-晶状体蛋白在各周龄正常大鼠晶状体上皮细胞及纤维部具有较高的表达。在8周龄、10周龄先天性白内障大鼠晶状体上皮细胞及纤维部可观察到与正常对照组相同的较强的免疫活性,而12周龄、14周龄鼠的白内障晶状体纤维部αB-晶状体蛋白的免疫活性明显低于正常对照组。结论在12周龄、14周龄先天性白内障大鼠晶状体纤维部,αB-晶状体蛋白的免疫活性减弱,在白内障形成过程中αB-晶状体蛋白可能被一些蛋白酶水解分化,从而促进白内障的形成。

αβ-晶状体蛋白在肿瘤中的研究进展

αβ-晶状体蛋白(Cryab)是热休克蛋白家族中最重要的基因之一。Cryab在体内广泛表达,具有独特的生物学特性,主要作为分子伴侣参与蛋白质的合成、折叠、积聚、装配、运输和降解。最新研究证实Cryab在肿瘤中高表达,可作为癌基因在恶性肿瘤发生、发展中发挥重要作用。与肿瘤患者的预后有着密切关系,预示其存在潜在的应用价值。本文就Cryab基因的结构和功能,及其在恶性肿瘤中的研究进展和作用机制做一综述,以期为深入研究Cryab在肿瘤中的功能提供科学依据。

一次力竭离心运动后大鼠骨骼肌αB-晶体蛋白的变化及针刺对其影响

目的:探讨一次力竭离心运动后大鼠骨骼肌αB-crystallin表达和血清CK的变化,及针刺对其的影响。方法:雄性SD大鼠分安静组、运动非针刺组与运动针刺组。运动组大鼠进行一次力竭离心运动,于运动后即刻对运动针刺组进行针刺处理。免疫组织化学的方法和比色法分析各组大鼠腓肠肌中αB-crystallin含量的变化和血清CK的值。结果:一次力竭离心运动后,运动针刺组大鼠αB-crystallin含量高于运动非针刺组大鼠(P<0.05)。运动针刺24h组血清CK显著低于运动即刻组(P<0.01);运动24h组与运动即刻组相比,血清CK值无显著性差异(P>0.05)。结论:1)针刺可促使运动诱导的αB-crystallin蛋白进一步表达,可能是针刺促进运动导致的骨骼肌损伤提前恢复的机制之一。2)针刺通过加强骨骼肌超微结构损伤修复促使血清CK含量提前恢复至24 h水平。

Sustained Contraction of Isolated Rabbit Thoracic Aortic Rings in Endothelial-dependent Manner Induced by βγ-CAT

In vertebrates, non-lens βγ-crystallins are widely expressed in various tissues and their functions are not well known. The molecular mechanisms of trefoil factors （TFFs）, which involved in mucosal healing and tumorigenesis, have remained elusive. βγ-CAT is a novel multifunctional protein complex of non-lens βγ-crystallin and trefoil factor from frog skin secretions. Here we report that βγ-CAT could induce sustained contraction of isolated rabbit aortic rings in dosage （2-35nmol/L） and endothelium dependent manners （P〈0.01 ）. In addition, in situ immunofluorescence indicated that positive TNF-α signals were mainly detected at the endothelial cell layer of βγ-CAT （25nmol/L） treated rings. Furthermore, βγ-CAT induced primary cultured rabbit thoracic aortic endothelial cells （RAECs） rapidly to release TNF-α. After βγ-CAT （25nmol/L） treated for 10 and 30min, the levels of the endothelial cells released TNF-ct were 34.17±5.10 pg/mL and 98.01±4.67 pg/mL （P〈0.01）, respectively. In conclusion, βγ-CAT could induce sustained contraction of isolated aortic rings, and the contractile effect might be partially explained by the release of TNF-α. These findings will give new insight into understanding the functions and physiological roles of non-lens βγ-crystallins and trefoil factors.

Identification of the preferentially targeted proteins by carbamylation during whole lens incubation by using radio-labelled potassium cyanate and mass spectrometry

AIMTo attempt to identify the primary targets of carbamylation in bovine lenses incubated under physiological condition.

外周血Cryab联合MRI检测对视神经脊髓炎的诊断价值

目的评价外周血αβ-晶状体蛋白(Cryab)联合MRI检测对视神经脊髓炎(NMO)的诊断价值。方法选取2019年1月至2020年2月长兴县人民医院收治的NMO患者53例作为NMO组,同期在本院门诊进行健康体检的健康志愿者50例作为对照组。采用Western blot法检测所有研究对象外周血Cryab表达水平,收集所有研究对象颅脑MRI图像,比较两组研究对象外周血Cryab表达水平及颅脑影像状况。分析外周血Cryab、颅脑MRI及两者联合检测诊断NMO的灵敏度与特异度,及外周血Cryab联合MRI检测与临床确诊结果的一致性。结果NMO组患者外周血Cryab表达水平为0.825±0.251,高于对照组的0.305±0.077,差异有统计学意义(P<0.05)。外周血Cryab对NMO诊断的灵敏度和特异度分别为0.774、0.860;MRI检测对NMO诊断的灵敏度和特异度分别为0.679、1.000;外周血Cryab联合MRI检测对NMO诊断的灵敏度和特异度分别为0.755、1.000。相比于单独检测,两者联合检测的灵敏度与特异度均得到较大提高,且与临床确诊结果的一致性良好(Kappa=0.749)。结论外周血Cryab联合MRI检测可以较准确地诊断NMO,能够为患者的临床诊治提供指导信息。

Computer construction and analysis of protein models of the mutant γD-crystallin gene

Background γD-crystallin plays an important role in human cataract formation. Being highly stable, γD-crystallin proteins are composed of two domains. In this study we constructed and analyzed protein models of the mutant γD-crystallin gene, which caused a special fasciculiform congenital cataract affecting a large Chinese family. Methods γD-crystallin protein structure was predicted by Swiss-Model software using bovine γD-crystallin as a template and Prospect software using human βb2-crystallin as a template. The models were observed with a Swiss-Pdb viewer.Results The mutant γD-crystallin structure predicted by the Swiss-Model software showed that proline23 was an exposed surface residue and P23T change made a decreased hydrogen bond distance between threonine23 and asparagine49. The mutant γD-crystallin structure predicted by the Prospect software showed that the P23T change exerted a significant effect on the protein’s tertiary structure and yielded hydrogen bonds with aspartic acid21, asparagine24, asparagine49 and serine74.Conclusion The mutant γD-crystallin gene has a significant effect on the protein’s tertiary structure, supporting that alteration of γ-crystallin plays an important role in human cataract formation.

Cataract-causing mutation S228P promotes βB1-crystallin aggregation and degradation by separating two interacting loops in C-terminal domain

β/γ-Crystallins are predominant structural proteins in the cytoplasm of lens fber cells and share a similar fold composing of four Greek-key motifs divided into two domains. Numerous cataract-causing mutations have been identified in various β/γ-crystallins, but the mech- anisms underlying cataract caused by most mutations remains uncharacterized. The S228P mutation in βB1- crystallin has been linked to autosomal dominant con- genital nuclear cataract. Here we found that the S228P mutant was prone to aggregate and degrade in both of the human and E. coli cells. The intracellular S228P aggregates could be redissolved by lanosterol. The S228P mutation modified the refolding pathway of βB1- crystallin by affecting the formation of the dimeric intermediate but not the monomeric intermediate. Compared with native βBl-crystallin, the refolded S228P protein had less packed structures, unquenched Trp fluorophores and increased hydrophobic exposure. The refolded S228P protein was prone to aggregate at the physiological temperature and decreased the protective effect of βB1-crystallin on βA3-crystallin. Molecular dynamic simulation studies indicated that the mutation decreased the subunit binding energy and modified the distribution of surface electrostatic potentials. More importantly, the mutation separated two interacting loops in the C-terminal domain, which shielded the hydrophobic core from solvent in native βB1-crystallin. These two interacting loops are highly conserved in both of the N- and C-terminal domains of all β/γ-crys- tallins. We propose that these two interacting loops play an important role in the folding and structural stability of β/γ-crystallin domains by protecting the hydrophobic core from solvent access.

Characterization of three transcripts encoding small heat shock proteins expressed in the codling moth, Cydia pomonella （Lepidoptera： Tortricidae）

Codling moth is a major pest of apples and pears worldwide. Increasing knowledge of how this insect responds to environmental stress will improve field and postharvest control measures used against it. The small heat shock proteins （sHsps） play a maj or role in cellular responses to environmental stressors. A degenerate oligonucleotide primer, designed against the conserved α-crystallin domain, was used in 3＇ rapid amplification of complementary DNA （cDNA） ends reactions to amplify transcripts encoding sHsps expressed in the codling moth cell line, Cp169, subjected to heat shock. Three full-length cDNAs were cloned from Cp169 cells that contained open reading frames encoding sHsps. The cDNA for CpHsp 19.8 was 795 bp encoding 177 amino acids. The cDNA for CpHsp 19.9 was 749 bp encoding 175 amino acids. The cDNA for CpHsp22.2 was 737 bp encoding 192 amino acids. Analysis of the protein sequences of the three CpHsps indicated the presence of 83 amino acids with homology to the α-crystallin domain. For each of the CpHsps, the α-crystallin domain was surrounded by divergent N- and C-terminal regions, consistent with the conserved structural features of sHsps. Real-time polymerase chain reaction, used to determine the expression patterns of each of the sHsps in different developmental stages of codling moth revealed the presence of transcripts in all stages tested. Consistent with characteristics of other sHsps, expression of CpHsp transcripts were greatly enhanced when insects were subjected to heat shock. The results of this research can be used as a guide to study the roles of sHsps in codling moth control using various post-harvest treatments.