Production of marker-free transgenic plants from mature tissues of navel orange using a Cre/loxP site-recombination system

Genetic transformation with mature material as the explants could shorten the transgenic period and avoid seed dependence compared with genetic transformation using the epicotyl seedling stem segments as the receptor. Here, we constructed an Agrobacterium tumefaciensmediated transformation for generation of marker-free transgenic plants from navel orange(Citrus sinensis Osbeck) mature stems using a CreloxP recombination system. To efficiently recover the regenerated buds from mature tissues, five recovery methods were compared: in vitro micrografting of 0.1-0.5(1-2 weeks), > 0.5 cm(3-4 weeks) and > 1 cm long lignified bud and in vitro micrografting of explants with a bud and rooting regenerated bud. The data showed that in vitro micrografting of > 1 cm long regenerated bud with expanded leaves after one month of continuous culture for lignification was the optimal solution for plant recovery from mature tissues. Transgenic plants without selectable marker genes were created from navel orange(Citrus sinensis Osbeck) tissue using a transformation vector PLI-35SPR1aCB containing a Cre/loxP system recombination together with genes encoding the selectable marker isopentenyl transferase(IPT) and an anti-bacterial peptide(PR1aCB).Using IPT positive selection, the transformation efficiency determined by PCR was 0.9%, and in total, 20 transgenic plants were obtained.Southern blotting confirmed further their transgenicity. PCR and sequencing analysis demonstrated that both the Cre and IPT genes had been successfully removed from the transgenic plants(deletion efficiency 100%). Over all, using Cre/loxP system recombination together with the IPT positive selection, marker-free transgenic plants can be recovered efficiently from mature tissues of navel orange(Citrus sinensis Osbeck), which provides a potential method for production of transgenic plants from citrus mature tissue.

Rapid Generation of Selectable Marker-Free Transgenic Rice with Three Target Genes by Co-Transformation and Anther Culture

The ＇double T-DNA＇ binary vector p13HSR which harbored two independent T-DNAs, containing hygromycin phosphotransferase gene （hpf） in one T-DNA region and three target genes （hLF, SB401, RZ10） in another T-DNA region, was used to generate selectable marker-free transgenic rice by Agrobacterium-mediated transformation. The regenerated plants with both the three target genes and the selectable marker gene hpt were selected for anther culture. RT-PCR analysis indicated that target genes were inserted in rice genomic DNA and successfully transcribed. It took only one year to obtain double haploid selectable marker-free transgenic plants containing the three target genes with co-transformation followed by anther culture technique, and the efficiency was 12.2%. It was also noted that one or two target genes derived from the binary vector were lost in some transgenic rice plants.

Breeding of Selectable Marker-Free Transgenic Rice Lines Containing AP1 Gene with Enhanced Disease Resistance

In order to obtain marker-free transgenic rice with improved disease resistance, the AP1 gene of Capsicum annuum and hygromycin-resistance gene （HPT） were cloned into the two separate T-DNA regions of the binary vector pSB130, respectively, and introduced into the calli derived from the immature seeds of two elite japonica rice varieties, Guangling Xiangjing and Wuxiangjing 9, mediated by Agrobacterium-mediated transformation. Many cotransgenic rice lines containing both the AP1 gene and the marker gene were regenerated and the integration of both transgenes in the transgenic rice plants was confirmed by either PCR or Southern blotting technique. Several selectable marker-free transgenic rice plants were subsequently obtained from the progeny of the cotransformants, and confirmed by both PCR and Southern blotting analysis. These transgenic rice lines were tested in the field and their resistance to disease was carefully investigated, the results showed that after inoculation the resistance to either bacterial blight or sheath blight of the selected transgenic lines was improved when compared with those of wild type.

Construction of Marker-Free GFP Transgenic Tobacco by Cre/lox Site-Specific Recombination System

Marker-free GFP transgenic tobacco plants were constructed based on Cre/lox site-specific recombination system. A GFP gene was introduced into the tobacco genome using the Bar gene as a linked selectable marker flanked by recombination sites in a directed orientation. The Bar gene expression box was subsequently excised from the plant genome by a strategy of Cre gene retransformation. After removal of the Cre-NPT Ⅱ locus by genetic segregation through self-cross, plants that incorporated only the GFP transgene were obtained. Transgenic tobacco plants mediated by Agrobacterium tumefaciens were obtained, which resisted herbicide Basta and GFP expressed well, then the Cre gene was subsequently introduced into 5 plants of them, respectively, by retransformation. The leaf disks from Cre transgenic plants were used to test the resistance to Basta on the medium with 8 mg L-1 of PPT. The results showed that few discs were able to regenerate normally, and the excision at 76-100% efficiency depended on individual retransformation events. Evidence for a precise recombination event was confirmed by cloning the nucleotides sequence surrounding the lox sites of the Basta sensitive plants. The result indicated that the excision event in the recombination sites was precise and conservative, without loss or alteration of any submarginal nucleotides of the recombination sites. Bar gene excised plants were selfpollinated to allow segregation of the GFP gene from the Cre-NPT Ⅱ locus. The progenies from self-pollinated plants were scored for Kan senstivity, then the segregation of GFP gene from Cre-NPT Ⅱ locus in the Kan senstive plants were confirmed by PCR analysis subsequently. Hence, constructing marker-free transgenic tobacco plants by Cre/lox sitespecific recombination system was reliable, and the strategy presented here should be applicable to other plants for the construction of marker-free transgenic plants as well.

Development of Marker-Free Transgenic Cry1Ab Rice with Lepidopteran Pest Resistance by Agrobacterium Mixture-Mediated Co-transformation

CrylAb gene was transformed into four rice varieties, Zhejing 22, Zhejing 27, Jiahua 1 and Xiushui 63 mediated by Agrobacterium-mixture co-transformation. Rice genotype had an important effect on callus induction and transformation efficiency. Different mixtures of Agrobacterium strains （EHA105 and EHA101） contained Hpt and CrylAb genes resulted in different frequencies of resistant calli. There was no correlation between the frequency of transformants with the ratio of the Agrobacterium strain mixture contained Hpt and CrylAb genes. A total of 509 transgenic plants were obtained from the four rice varieties, and 272 T2 progenies were analyzed for CrylAb and Hpt genes. PCR analysis revealed that 412 regenerated plants were Hpt positive （80.94%）, 62 plants were also CrylAb co-transformants （15.05% in total frequency）, and 42 plants among the 272 T2 progenies were CrylAb positive but Hpt negative. This suggests that marker-free transgenic plants could be produced by co-transformation mediated by mixed Agrobacterium strains with the selectable marker gene and target gene Southern blot analysis of five independent marker-free T2 transgenic lines co-transformed from Zhejing 22 showed that CrylAb gene had been inserted into rice genome with a single copy. The transgenic plants showed significantly stronger resistance to lepidopteron than the non-transgenic plants under no application of insecticides against lepidopteron.

Genetic and agronomic traits stability of marker-free transgenic wheat plants generated from Agrobacterium-mediated co-transformation in T2 and T3 generations

Genetically modified wheat has not been commercially utilized in agriculture largely due to regulatory hurdles associated with traditional transformation methods. Development of marker-free transgenic wheat plants will help to facilitate biosafety evaluation and the eventual environmental release of transgenic wheat varieties. In this study, the marker-free transgenic wheat plants previously obtained by Agrobacterium-mediated co-transformation of double T-DNAs vector were identified by fluorescence in situ hybridization(FISH) in the T1 generation, and their genetic stability and agronomic traits were analyzed in T2 and T3 generations. FISH analysis indicated that the transgene often integrated into a position at the distal region of wheat chromosomes. Furthermore, we show that the GUS transgene was stably inherited in the marker-free transgenic plants in T1 to T3 generations. No significant differences in agronomic traits or grain characteristics were observed in T3 generation, with the exception of a small variation in spike length and grains per spike in a few lines. The selection marker of bar gene was not found in the transgenic plants through T1 to T3 generations. The results from this investigation lay a solid foundation for the potential application of the marker-free transgenic wheat plants achieved through the co-transformation of double T-DNAs vector by Agrobacterium in agriculture after biosafty evaluation.

Development and drought tolerance assay of marker-free transgenic rice with OsAPX2 using biolistic particle-mediated co-transformation

Abiotic stresses such as drought, salinity, and low temperature cause–losses in rice production worldwide. The emergence of transgenic technology has enabled improvements in the drought resistance of rice plants and helped avert crop damage due to drought stress.Selectable marker genes conferring resistance to antibiotics or herbicides have been widely used to identify genetically modified plants. However, the use of such markers has limited the public acceptance of genetically modified organisms. Marker-free materials (i.e., those containing a single foreign gene) may be more easily accepted by the public and more likely to find common use. In the present study, we created marker-free drought-tolerant transgenic rice plants using particle bombardment. Overall, 842 T_0plants overexpressing the rice ascorbate peroxidase-coding gene OsAPX2 were generated. Eight independentmarker-free lines were identified from T_1 seedlings using the polymerase chain reaction.The molecular characteristics of these lines were examined, including the expression level,copy number, and flanking sequences of OsAPX2, in the T_2 progeny. A simulated drought test using polyethylene glycol and a drought-tolerance test of seedlings confirmed that the marker-free lines carrying OsAPX2 showed significantly improved drought tolerance in seedlings. In the field, the yield of the wild-type plant decreased by 60% under drought conditions compared with normal conditions. However, the transgenic line showed a yield loss of approximately 26%. The results demonstrated that marker-free transgenic lines significantly improved grain yield under drought-stressed conditions.

Efficiencies of Generating Selectable Marker-Free Transgenic Rice with Different Transformation Methods

To study the efficiency of generating selectable marker-free （SMF） transgenic rice, two transformation methods were employed for four rice varieties （Wuxiangjing 9, Longtefu, Xieqingzao and Zhenshan 97）. One method is by using a single twin T-DNA binary vector pYH592 in one Agrobacterium strain, which is composed of two separate T-DNA regions （one carrying an antisense Wx gene and the other carrying a HPTgene）. The other one, named as two-strain/two-vector system, is by using two separate binary vectors in two separate Agrobacterium cultures. The results indicated that the average co-transformation frequencies of the antisense Wx gene and the HPT gene were 10.1% and 45.0%, respectively, for the four rice varieties. And the SMF transgenic plants selected from the offsprings of co-transformants were 55.6% and 60.0% in the two-strain/two-vector and twin T-DNA vector binary systems, respectively.

低温与无水胁迫下凡纳滨对虾肌肉品质劣变标记蛋白识别

【目的】探明凡纳滨对虾(Litopenaeus vannamei)保活流通过程中低温和无水双重胁迫诱导肌肉品质劣变与差异表达蛋白之间的相关性,识别品质劣变的潜在标记蛋白。【方法】在模拟的海水环境中[溶解氧质量浓度为7.2 mg/L,温度控制在(12±1)℃]观察对虾在低温和无水胁迫下的生理反应,通过串联质谱标签蛋白质组学方法,分析环境胁迫导致的肝胰腺蛋白质组显著差异性变化,并将其与肌肉品质进行相关性分析。【结果】与正常对照组相比,低温组和低温+无水组分别鉴定了33和44个显著差异蛋白质(DEPs),这些蛋白质大多在溶酶体、糖酵解或糖异生、黏附等通路显著富集(P<0.05),同时胰蛋白酶-1、二肽基肽酶显著上调(P<0.05),而磷酸丙糖异构酶和醛脱氢酶显著下调(P<0.05)。此外,颜色和质构指标的变化与微管蛋白、凝溶胶蛋白、层黏连蛋白、内源性蛋白酶和代谢酶表达水平显著相关。【结论】本研究初次探明肝胰腺DEPs与肌肉品质间的内在联系,识别的典型DEPs可作为品质劣变的潜在标志蛋白,为监测无水运输期间凡纳滨对虾肌肉品质劣变提供分子靶标。

无标记运动捕捉系统在临床步态分析上的研究进展

步态分析是临床研究的重要组成部分,传统的三维步态分析由于设备成本高、专业技术要求高等原因难以广泛应用。随着计算机视觉技术的发展,无标记运动捕捉系统的精确度得到极大提升,无需标记、成本较低的优势逐渐显现,并被应用于步态分析,但由于研究人员和临床医生缺乏对该系统的整体了解,使得该技术尚不能得到广泛推广,本综述拟对无标记运动捕捉系统在临床步态分析上的应用进展进行回顾,分析目前各项技术的优势和局限性,展望无标记运动捕捉系统在临床步态分析上的发展方向,为今后无标记运动捕捉系统在临床上的推广使用提供了研究思路。

食管癌患者循环肿瘤细胞与临床特征和全身炎症标志物的关系及其预后价值

目的构建一个列线图模型来评估食管癌(EC)患者根治性手术(RS)后的生存率,并通过限制性立方样条(RCS)来评估循环肿瘤细胞(CTC)、全身炎症标志物和预后之间的非线性关系。方法测定RS后采集的500例EC患者血液中CTC计数,计算系统免疫炎症指数(SII)、中性粒细胞与淋巴细胞和血小板的比值(NLPR)、全身炎症聚集指数(AISI)和全身炎症反应指数(SIRI),分析临床数据与这些指标的相关性。评估CTC计数和全身炎症标志物对总生存期(OS)和无进展生存期(PFS)的预测价值。结果CTC与临床特征(新辅助治疗、术前合并症、病理分级、脉管侵犯、神经侵犯和肿瘤大小)和炎症标志物(SII、NLPR、SIRI、AISI)存在较强的相关性。单因素和多因素Cox回归分析显示:新辅助治疗(P=0.031)、术前合并症(P=0.028)、治疗方式(P<0.001)、病理分级(P=0.006)、脉管侵犯(P=0.012)、神经侵犯(P=0.012)、SII(P<0.001)、NLPR(P=0.008)、AISI(P<0.001)、CTC(P<0.001)为独立的预后影响因素。T分期(P=0.036)、N分期(P=0.002)和脉管侵犯(P<0.001)与PFS有相关性。RCS图显示CTC、SII、NLPR、SIRI和AISI与预后呈非线性关系。Kaplan-Meier生存曲线显示,CTC、SII、NLPR、SIRI和AISI值较低的患者OS和PFS较长(P<0.05)。结论CTC、SII、NLPR和AISI可能是EC患者行RS的临床预后的有力指标,结合这些因素的列线图和RCS有助于临床实践中患者预后的个体化判断。

安罗替尼联合IP方案治疗进展/复发小细胞肺癌临床研究

目的探讨安罗替尼联合IP方案(伊立替康+顺铂)治疗进展/复发小细胞肺癌(SCLC)的临床效果及其作用机制。方法选取医院2019年6月至2021年6月收治的进展/复发SCLC患者97例,按随机数字表法分为对照组(48例)和观察组(49例),两组患者均予IP方案治疗,观察组患者加服盐酸安罗替尼胶囊。两组均以28 d为1个周期,连续治疗2个周期,随访20个月。结果观察组患者的疾病控制率显著高于对照组(P<0.05);观察组患者治疗后的血清癌胚抗原(CEA)、神经元特异性烯醇化酶(NSE)、细胞角蛋白19片段(Cyfra21-1)水平及肿瘤代谢体积(MTV)、血容量(BV)、血流量(BF)均显著低于对照组(P<0.05);观察组患者中位无进展生存期(PFS)显著长于对照组(7.5个月比5.5个月,P<0.05);两组患者的不同等级不良反应发生率、生存率均无显著差异(P>0.05)。结论安罗替尼联合IP方案治疗进展/复发SCLC,可降低患者的肿瘤负荷,延长PFS,机制可能与调节肿瘤标志物和改善血流灌注指标有关。

大黄炭炮制过程中“增效”和“减毒”潜在质量标志物的变化规律研究

目的:通过筛选大黄炭的潜在质量标志物,分析大黄炭炮制过程中潜在质量标志物的变化规律,为大黄炭炮制机理研究与炮制终点判断提供参考。方法:本研究基于经典文献与网络药理学分析,初步筛选大黄炭的潜在质量标志物。以LPS诱导的HUVEC细胞作为大黄炭“凉血化瘀”功效的体外评价模型,进一步验证大黄炭的潜在质量标志物。使用色差仪对大黄炭的颜色特征进行量化,分析大黄炭炮制过程中潜在质量标志物与颜色变化的关联性。结果:大黄炭的潜在质量标志物可分为两类:结合蒽醌与番泻苷为一类,随炮制程度增加而递减,可能与大黄制炭后泻下作用减弱有关;游离蒽醌、没食子酸、5-HMF为另一类,随炮制程度增加而先增后减,可能与大黄制炭后凉血化瘀作用增加有关。结论:大黄炭中结合蒽醌可作为潜在的“减毒”质量标志物,游离蒽醌可作为潜在的“增效”质量标志物。

白蛋白紫杉醇与卡铂联合替雷利珠单抗治疗晚期非小细胞肺癌的效果

目的探讨白蛋白紫杉醇与卡铂联合替雷利珠单抗治疗晚期非小细胞肺癌(non-small cell lung cancer,NSCLC)的效果及对肿瘤标志物、无病生存期(disease-free survival,DFS)的影响。方法回顾性分析82例晚期NSCLC患者的临床资料,对照组(n=40)给予白蛋白紫杉醇联合卡铂治疗,观察组(n=42)在对照组治疗的基础上给予替雷利珠单抗治疗,比较2组的临床疗效、血清相关因子[胃泌素释放肽前体(pro-gastrin-releasing peptide,ProGRP)、肿瘤坏死因子-α(tumour necrosis factor-α,TNF-α)]、肿瘤标志物[糖类抗原125(carbohydrate antigen 125,CA125)、癌胚抗原(carcinoembryonic antigen,CEA)、神经元特异性烯醇化酶(neuron-specific enolase,NSE)、细胞角蛋白19片段抗原21-1(cytokeratin-19-fragment CYFRA21-1,CYFRA21-1)]、免疫功能、不良反应发生率、DFS和总生存率。结果观察组疾病缓解率(response rate,RR)高于对照组(73.81%vs.52.50%),P<0.05。治疗后,2组血清ProGRP、TNF-α、CA125、CEA、NSE和CYFRA21-1水平均降低(P<0.05);且观察组血清ProGRP、TNF-α、CA125、CEA、NSE和CYFRA21-1水平均显著低于对照组(P<0.05);2组表面抗原分化簇3受体(differentiation cluster 3 receptor,CD3+)、表面抗原分化簇4受体(differentiation cluster 4 receptor,CD4+)、CD4+/表面抗原分化簇8受体(differentiation cluster 8 receptor,CD8+)水平升高,CD8+水平降低(P<0.05),且观察组CD3+、CD4+、CD4+/CD8+均显著高于对照组,CD8+显著低于对照组(P<0.05)。2组不良反应发生率比较差异无统计学意义。随访6个月,观察组复发(转移)率低于对照组(16.67%vs.37.50%),DFS长于对照组,总生存率高于对照组(80.95%vs.60.00%),P<0.05。结论白蛋白紫杉醇与卡铂联合替雷利珠单抗治疗晚期NSCLC的效果显著,可抑制肿瘤新生血管形成,降低肿瘤标志物,提高免疫功能和延长DFS。

幕下弥漫性胶质瘤患者预后相关因素分析

目的:探究幕下弥漫性胶质瘤预后的影响因素。方法:收集2016年1月—2020年6月天津市环湖医院经手术治疗的35例幕下胶质瘤患者的临床资料,分析年龄、性别、肿瘤切除程度、α地中海贫血伴智力低下综合征X染色体相关蛋白(ATRX)基因突变、O6-甲基鸟嘌呤-DNA-甲基转移酶(MGMT)启动子区甲基化对幕下弥漫性胶质瘤患者的总生存期(OS)及无进展生存期(PFS)的影响。结果:幕下弥漫性胶质瘤平均PFS为13.28个月(95%CI:10.14~16.42),平均OS为15.97个月(95%CI:12.43~19.52);肿瘤全切或次全切、术后卡氏功能状态评分标准(KPS评分)≥70分、MGMT甲基化及ATRX突变是PFS预后良好的因素;肿瘤全切或次全切、术后KPS评分≥70分、年龄<48岁及ATRX突变是OS预后良好的因素。结论:年龄小、肿瘤切除范围大、术后KPS评分≥70分、ATRX突变的幕下弥漫性胶质瘤患者术后有更长的生存期。

基于Label-free技术的非小细胞肺癌蛋白质差异研究

目的 基于非小细胞肺癌(non-small-cell lung cancer,NSCLC)及与其配对的非癌性邻近组织(non-cancerous adjacent tissues,NATs)的蛋白质组学分析,寻找NSCLC诊断相关蛋白标志物。方法 应用非标记定量蛋白组学(LFP)技术,以NSCLC患者配对的NATs为对照,对5例NSCLC患者进行癌组织蛋白质组学分析。以差异倍数>1.5(上调)或<0.67(下调)且P<0.05为标准筛选差异蛋白。应用String网站和R语言对差异蛋白进行基因本体论(gene ontology,GO)分析、京都基因和基因组百科全书(Kyoto Encyclopedia of Genes and Genomes,KEGG)分析,为进一步研究提供良好基础。结果 本研究发现差异蛋白共644个,其中339个蛋白表达上调,305个蛋白表达下调。PCA结果显示,差异蛋白可明显区分NSCLC与NATs。GO分析结果表明,差异蛋白大多以细胞外泌体的形式存在且主要富集于调节胞外分泌、胞外分泌、骨髓细胞激活参与免疫反应等的生物学过程以及钙粘着蛋白绑定、细胞外基质绑定等的分子功能。KEGG分析结果显示,差异蛋白主要富集在抗坏血酸和醛酸代谢、组氨酸代谢、蛋白质消化吸收、丙酮酸代谢等通路(P<0.05)。结论 NSCLC与NATs存在明显差异,可为发现NSCLC新型标志物提供线索。

血清肿瘤标志物单独以及联合检测在原发性肝癌中的诊断价值研究

目的 分析血清肿瘤标志物单独以及联合检测在原发性肝癌中的诊断价值。方法 回顾性选取2020年2月—2022年2月曹县人民医院疑似原发性肝癌患者50例的临床资料。运用化学发光酶免分析方法测定血清胆碱酯酶(cholinesterase, CHE)、γ-谷氨酰转肽酶(gamma-glutamyl transpeptidase, GGT)、α-L-岩藻糖苷酶(α-L-fucosidase, AFU)、甲胎蛋白(alpha-fetoprotein, AFP)、铁蛋白(ferritin, SF)等肿瘤标志物水平。统计分析肿瘤标志物单独与联合检测的阳性情况,并统计分析肿瘤标志物单独与联合检测的诊断效能。以病理学检查为金标准。结果 AFP、SF的灵敏性、准确性均高于CHE、GGT、AFU,差异有统计学意义(P<0.05)。联合检测灵敏性为100.00%,特异性为100.00%,准确性为100.00%,阳性预测值为100.00%,阴性预测值为100.00%,联合检测灵敏性、准确性均高于CHE、GGT、AFU、AFP、SF,差异有统计学意义(P<0.05),联合检测的阴性预测值高于AFP、SF,差异有统计学意义(P<0.05)。结论 血清肿瘤标志物水平在原发性肝癌诊断中的应用价值高,联合检测较单独检测的诊断效能高。

扶正祛邪养阴方辅助化疗治疗晚期气阴两虚型非小细胞肺癌患者的疗效

目的:探讨扶正祛邪养阴方辅助化疗治疗晚期气阴两虚型非小细胞肺癌(NSCLC)患者的疗效。方法:选取2020年1月至2021年9月德驭医疗马鞍山总医院收治的晚期NSCLC患者120例作为研究对象,按照随机数字表法随机分为对照组和观察组,每组60例,对照组给予多西他赛+顺铂化疗,观察组在对照组基础上加用扶正祛邪养阴方治疗。比较2组患者间近期疗效,中医症状积分,肿瘤标志物血清糖类抗原125(CA125)、细胞角质素片段抗原21-1(CYFRA21-1)和癌胚抗原(CEA),免疫功能自然杀伤细胞(NK)、细胞毒T细胞(Tc)、和调节性T细胞(Treg)比例,生命质量(卡诺夫斯凯计分评分),不良反应及1年无进展生存期、无进展生存率及1年总生存率。结果:2组患者间疾病控制率、1年无进展生存期、无进展生存率及1年总生存率比较差异无统计学意义(P>0.05);治疗后,观察组中医症状积分、肿瘤标志物(CA125、CYFRA21-1和CEA)、免疫功能(NK、Tc、和Treg比例)、卡诺夫斯凯计分评分和对照组差异均有统计学意义(均P<0.05),不良反应(胃肠道反应、骨髓抑制和肝功能异常)发生率显著低于对照组(P<0.05)。结论:扶正祛邪养阴方辅助化疗治疗晚期气阴两虚型NSCLC患者,能有效缓解临床症状,降低肿瘤标志物水平,提高免疫功能,降低不良反应发生率。

无抗性选择标记的转高赖氨酸蛋白(LRP)基因籼稻恢复系的获得

将四棱豆中高赖氨酸含量蛋白基因转移到水稻恢复系R893中,获得了较好表达高赖氨酸含量蛋白基因、且无抗生素选择标记的籼稻恢复系C28。赖氨酸分析结果表明,C28为3.752 mg/g,对照R893为3.503 mg/g;杂交组合准S/C28为3.338 mg/g,对照准S/R893为3.175 mg/g。转基因水稻的赖氨酸含量都有所提高。但C28的结实率为76.37%,而R893为78.56%,转基因恢复系略低于对照;准S/C28为76.63%,对照准S/R893为89.35%,转基因的杂种极显著地低于对照。

无选择标记转基因植物的培育

植物转基因研究中通常都要使用选择标记基因来筛选转化细胞并获得转基因植株。但是当转基因植株育成后,选择标记基因就失去了存在的意义。为了消除由选择标记基因引起的安全性隐患,人们发展了一些培育无选择标记转基因植物的策略。这些策略主要包括共转化、位点特异性重组和转座子转座等。去除选择标记基因将促进公众对转基因作物的接受。评述了无选择标记转基因植物的研究进展。