内含子的位置不影响转基因的表达

内含子在转基因动物的基因表达中具有重要作用,以乳清酸蛋白（ＷＡＰ）基因５′区为调控序列,人基因组Ｇ－ＣＳＦ基因为目的片段,将ＷＡＰ基因第一内含子插入Ｇ－ＣＳＦ基因５′端,构建成转基因动物乳腺表达载体。将其直接注射到小鼠乳腺,在泌乳期表达出人Ｇ－ＣＳＦ。表明内含子在５′端的位置不影响转基因的表达,同时也表明内含子对表达有一定的作用。     

转基因动物与基因表达调控的研究

十余年来,随着转基因技术的快速发展,基因表达调控的转基因研究已逐渐开展。本文在下列几方面介绍了转基因动物技术在基因表达调控中的应用。转基因动物可作为在体内研究外源基因表达调控的“反应器”,例如研究酶对底物作用的种属特异性。可以精确研究ＤＮＡ顺式作用序列,探讨包括改变基因表达在内的组织和阶段特异性表达,增强子、内含子和核基质附着区的调节作用以及各基因间相互作用。转基因动物可研究发育中的时、空调节（如     

转基因动物与基因表达调控的研究

十余年来,随着转基因技术的快速发展,基因表达调控的转基因研究已逐渐开展。本文在下列几方面介绍了转基因动物技术在基因表达调控中的应用。转基因动物可作为在体内研究外源基因表达调控的“反应器”,例如研究酶对底物作用的种属特异性。可以精确研究ＤＮＡ顺式作用序列,探讨包括改变基因表达在内的组织和阶段特异性表达,增强子、内含子和核基质附着区的调节作用以及各基因间相互作用。转基因动物可研究发育中的时、空调节（如β－珠蛋白基因和同源异形盒基因）以及基因多级调节系统。通过同源重组得到基因缺陷动物（基因敲除动物）可探讨目的基因突变所致的异常表型以研究基因功能与调控。     

不同方向内含子对重组CHO细胞中神经生长因子表达的影响

为了研究不同方向的嵌合体内含子对重组神经生长因子 (Nerve growth factor,NGF) 基因表达的影响,以人β-珠蛋白第一内含子5?端剪接序列和人免疫球蛋白重链可变区内含子3?端剪接序列组合而成的嵌合体内含子作为研究对象,在NGF基因5?端插入不同方向的嵌合体内含子,构建含不同方向内含子的NGF基因表达载体。转染至CHO细胞后,G418筛选稳定转染的细胞,荧光定量PCR、ELISA和Western blotting检测不同载体NGF基因的表达情况。结果显示内含子可以大幅度提高NGF基因的表达,且正向内含子对NGF基因表达的增强作用无论是在mRNA水平还是在蛋白水平都要高于反向内含子。所以内含子能够提高外源NGF基因的表达,且内含子调控转基因表达具有方向性。     

不同方向内含子对重组CHO细胞中神经生长因子表达的影响（英文）

为了研究不同方向的嵌合体内含子对重组神经生长因子(Nerve growth factor,NGF)基因表达的影响,以人β-珠蛋白第一内含子5'端剪接序列和人免疫球蛋白重链可变区内含子3'端剪接序列组合而成的嵌合体内含子作为研究对象,在NGF基因5'端插入不同方向的嵌合体内含子,构建含不同方向内含子的NGF基因表达载体。转染至CHO细胞后,G418筛选稳定转染的细胞,荧光定量PCR、ELISA和Western blotting检测不同载体NGF基因的表达情况。结果显示内含子可以大幅度提高NGF基因的表达,且正向内含子对NGF基因表达的增强作用无论是在mRNA水平还是在蛋白水平都要高于反向内含子。所以内含子能够提高外源NGF基因的表达,且内含子调控转基因表达具有方向性。     

提高转基因表达水平的策略

随着转基因相关技术的发展,转基因动物技术在许多方面得到了成功应用.但外源基因在体内的表达仍然难以预测,特别是大动物的转基因,由于制备效率低下,因而难以筛选出足够的高表达的阳性动物数.基因表达调控研究对提高外源基因在动物体内的表达水平提供了一些新手段,本就避免转基因的位置效应、控制外源基因在动物宿主基因组中的整合、提高转基因的表达效率、构建转基因载体和使用外源基因需要注意的问题等进行综述.     

内含子对真核基因表达调控的影响

大多数真核基因都含有非编码的间隔序列--内含子,根据剪接机制的不同,可将内含子分为3类:真核mRNA内舍子、自我剪接内含子和真核tRNA内含子.在多数情况下,真核mRNA内含子的存在可以提高基因的表达水平.因为其剪接过程会影响mRNA新陈代谢的多个阶段,包括转录、RNA编辑、pre-mRNA的加工、mRNA的出核运输、翻译和无义衰变等.真核mRNA内含子在真核生物基因表达调控中起着重要的作用,是转基因研究中提高外源基因表达的重要元件之一.就真核mRNA内含子的特性、剪接机制及其对真核基因表达调控的影响作一概述.     

提高转基因表达策略研究进展

随着转基因技术在各个应用领域的深入和发展 ,转基因沉默现象已引起越来越多人的关注。在介绍转基因沉默的概念、分子机理的基础上 ,着重对提高转基因表达的方法、策略及其研究进展进行综述。分别阐述内含子、组织特异性启动子、增强子、定点整合、DNA大片段、反式作用因子以及基因组调控元件核基质附着区对转基因表达的影响。为克服转基因失活、提高转基因的表达效率提供理论依据。     

Ⅲ类内含子及其对基因表达的影响

内含子是指断裂基因中的非编码区序列。根据内含子的核苷酸序列和RNA潜在折叠方式不同,可分成四种类型：Ⅰ类内含子、Ⅱ类内含子、Ⅲ类内含子和Ⅳ类内含子。Ⅲ类内含子为真核细胞前mRNA中的内含子。它可以启动某些基因的表达,影响基因的表达量;增加mRNA分子的稳定性;并通过选择性剪接调控基因的表达。Ⅲ类内含子可以提高转基因动物基因的表达效率。因此,基因工程中,为了提高表达效率,是选用基因组基因还是cDNA基因,应视具体基因而定。     

水稻OsBP-73基因表达需要其内含子参与

该实验室以前的研究表明,水稻OsBP-73基因含有2个外显子和1个长度为2 471 bp的内含子.该文报告用OsBP-73基因ATG翻译起始密码子(在第1外显子中)上游序列(1- 818～ 215)与GUS基因构成嵌合质粒pRSSl,将该质粒转化水稻后,在抗性愈伤组织和转基因植株中未能检测到GUS基因的表达.只有用含有完整的内含子及其上游序列(1 818～ 2 844)与GUS基因构成嵌合质粒(p13GNF)时,才能在p13GNF的转基因抗性愈伤组织和植株中检测到GUS基因的表达.实验还证明,单是内含子序列并不能驱动GUS基因在转基因水稻中表达.由此推测:OsBP-73基因的启动子序列驱动基因表达时,需要基因内含子的参与.     

Distinct roles of the first introns on the expression of Arabidopsis profilin gene family members

Profilin is a small actin-binding protein that regulates cellular dynamics of the actin cytoskeleton. In Arabidopsis (Arabidopsis thaliana), five profilins were identified. The vegetative class profilins, PRF1, PRF2, and PRF3, are expressed in vegetative organs. The reproductive class profilins, PRF4 and PRF5, are mainly expressed in pollen. In this study, we examined the role of the first intron in the expression of the Arabidopsis profilin gene family using transgenic plants and a transient expression system. In transgenic plants, we examined PRF2 and PRF5, which represent vegetative and reproductive profilins. The expression of the PRF2 promoter fused with the beta-glucuronidase (GUS) gene was observed in the vascular bundles, but transgenic plants carrying the PRF2 promoter-GUS with its first intron showed constitutive expression throughout the vegetative tissues. However, the first intron of PRF5 had little effect on the reporter gene expression pattern. Transgenic plants containing PRF5 promoter-GUS fusion with or without its first intron showed reproductive tissue-specific expression. To further investigate the different roles of the first two introns on gene expression, the first introns were exchanged between PRF2 and PRF5. The first intron of PRF5 had no apparent effect on the expression pattern of the PRF2 promoter. But, unlike the intron of PRF5, the first intron of PRF2 greatly affected the reproductive tissue-specific expression of the PRF5 promoter, confirming a different role for these introns. The results of a transient expression assay indicated that the first intron of PRF1 and PRF2 enhances gene expression, whereas PRF4 and PRF5 do not. These results suggest that the first introns of profilin genes are functionally distinctive and the first introns are required for the strong and constitutive gene expression of PRF1 and PRF2 in vegetative tissues.     

TPO内含子Ⅴ可显著增强人血小板生成素基因在乳腺细胞中的表达

人血小板生成素（thrombopoietin,TPO）基因组包括6个外显子和5个内含子,内含子在其表达过程中可能扮演着重要作用.为了研究人TPO基因组中不同内含子对TPO表达的影响,构建可在转基因动物乳腺中高水平表达人TPO的乳腺特异性表达质粒.本研究以65 kb的山羊β-casein启动子为调控元件,构建了包括人TPO cDNA(pTPOA)、TPO intronⅠ-TPO cDNA (pTPOB)、ΔTPO intronⅠ-TPO cDNA (pTPOC)、TPO intronⅤ-TPO cDNA (pTPOD)和TPO gDNA (pTPOE)等5种TPO乳腺特异性表达质粒,并在人乳腺细胞HC-11细胞上进行了瞬间表达研究.在转染48 h后,通过双抗体夹心的ELISA方法定量分析上述质粒在HC-11细胞上的表达水平.结果表明,含有内含子Ⅴ的 pTPOD的表达量最高,而含有整个基因组TPO的pTPOE表达水平最低.为了进一步证实pTPOD可在乳腺细胞中高水平表达,将pTPOD经脂质体包埋后注射到泌乳期山羊的乳腺中.结果显示,在山羊乳汁中可连续14 d检测到人TPO的表达.上述实验证实,人TPO基因组中的内含子V可显著提高TPO在HC-11细胞内的表达水平,并提示内含子Ⅴ中可能含有特殊的调控序列.     

Prevalence of intron gain over intron loss in the evolution of paralogous gene families

The mechanisms and evolutionary dynamics of intron insertion and loss in eukaryotic genes remain poorly understood. Reconstruction of parsimonious scenarios of gene structure evolution in paralogous gene families in animals and plants revealed numerous gains and losses of introns. In all analyzed lineages, the number of acquired new introns was substantially greater than the number of lost ancestral introns. This trend held even for lineages in which vertical evolution of genes involved more intron losses than gains, suggesting that gene duplication boosts intron insertion. However, dating gene duplications and the associated intron gains and losses based on the molecular clock assumption showed that very few, if any, introns were gained during the last ~100 million years of animal and plant evolution, in agreement with previous conclusions reached through analysis of orthologous gene sets. These results are generally compatible with the emerging notion of intensive insertion and loss of introns during transitional epochs in contrast to the relative quiet of the intervening evolutionary spans.     

Expression in transgenic tobacco of the bacterial neomycin phosphotransferase gene modified by intron insertions of various sizes

A plant selectable marker gene consisting of cauliflower mosaic virus expression signals and the proteincoding sequence of bacterial neomycin phosphotransferase was modified by insertion of an intron sequence from a storage protein gene, phaseolin. Correct and efficient splicing of the resulting mosaic RNA was observed in transgenic tobacco plants. The insertion of various linkers or gradual increase of intron size by addition in both orientations of internal intron sequences from another plant gene (parsley, 4-coumarate ligase) had little or no effect on the precision of slicing. The gene activity measured by selectability assay in the protoplast transformation showed that only introns enlarged to 1161 bases and longer caused decreased selectability. The suitability of such mosaic marker genes for studies of RNA splicing, DNA recombination and early events after infection of plants with Agrobacterium is discussed.