PTIP相关蛋白1在小鼠睾丸发育过程中的表达及定位

目的探索PTIP相关蛋白1(PTIP associated protein 1,PA1)在小鼠睾丸发育过程中的表达定位。方法采用RTPCR、实时定量PCR和免疫组织化学方法,对PA1在小鼠睾丸不同发育阶段的表达及定位进行检测。结果 RT-PCR和实时定量PCR结果显示,PA1 m RNA在1w、2w、4w、8w、12w、18w和24w的小鼠睾丸中均有表达,且其表达量在2w时达到最高峰,在小鼠性成熟(8w)以后,PA1的表达量趋于平稳。ABC法免疫组织化学染色显示PA1在1w、2w、4w和8w小鼠睾丸各级生精细胞、支持细胞和间质细胞的胞核中均有表达,免疫荧光双标进一步确定PA1表达于支持细胞和间质细胞。结论 PA1可能在维持生精细胞的正常分化及调节睾丸内分泌的平衡中起重要作用。     

丝氨酸/精氨酸蛋白特异激酶SRPK2在小鼠睾丸组织中的表达及意义

目的通过研究丝氨酸/精氨酸蛋白特异激酶2(serine/arginine-rich protein specific kinase 2,SRPK2)基因mRNA及其编码蛋白产物在小鼠睾丸组织中的表达特征,探讨该基因在精子发生过程中的作用及意义。方法分别采用半定量逆转录聚合酶链反应(RT-PCR)和蛋白免疫印迹杂交(Western blotting)分析该基因mRNA及蛋白产物在小鼠多种组织中的表达;利用实时定量PCR(real-time quantitative PCR)分析SRPK2 mRNA在不同发育阶段小鼠睾丸组织中的差异表达;应用免疫组织化学染色和间接免疫荧光技术观察SRPK2蛋白在小鼠曲精小管中的细胞定位和生精细胞内的亚细胞定位。结果半定量RT-PCR和Western blotting分析显示SRPK2 mRNA和蛋白在小鼠睾丸组织中均大量表达;实时定量PCR分析发现SRPK2 mRNA在5周及8周龄雄性小鼠睾丸组织中显著表达,具有明显的阶段特异性表达特征。免疫组织化学染色结果表明SRPK2蛋白阳性着色主要位于曲精小管中的长形精子细胞核;间接免疫荧光分析显示SRPK2蛋白定位于长形精子细胞核表面。结论 SRPK2基因在小鼠睾丸组织中大量表达,并且具有显著的阶段特异性表达特征和明确的细胞核定位,极有可能在小鼠精子发生的变态成形期参与mRNA前体分子的剪接过程,其作用机制值得进一步深入研究。     

检控蛋白Rad17在小鼠睾丸精子发生过程中的表达及其磷酸化变化

Rad17是细胞周期检控点信号转导过程中的一个关键检控蛋白,在DNA损伤检控和DNA复制检控中具有重要功能。但Rad17在细胞减数分裂中的检控作用还不是很清楚。因细胞减数分裂在睾丸组织中非常活跃,应用Western印迹检测Rad17在不同发育时期的小鼠睾丸组织中的表达及其磷酸化水平,并应用免疫组化的方法检测小鼠睾丸组织不同时期生殖细胞内Rad17的表达变化。结果显示Rad17在小鼠睾丸组织内高表达,而在肝、肾等组织中表达水平较低;Rad17在不同周龄的小鼠睾丸组织中均高水平表达,但在4周龄以后的小鼠睾丸组织中其磷酸化水平明显升高;免疫组化结果显示Rad17在精原细胞、精母细胞的细胞核中高表达,但在成熟精子细胞中消失。这些结果提示Rad17在小鼠睾丸生殖细胞减数分裂过程中也起重要检控作用。     

环境高温促进猪睾丸Apaf-1和Caspase-9的表达

高温热应激条件下,凋亡蛋白表达量升高,生殖细胞凋亡增加。凋亡蛋白酶活化因子1（apoptosis protease activating factor 1,Apaf-1）和凋亡蛋白酶活化起始者含半胱氨酸的天冬氨酸蛋白水解酶9,(cysteine aspartic acid specific protease 9, Caspase-9）是细胞凋亡内源途径中的重要调节蛋白,热应激条件下猪睾丸Apaf-1和Caspase 9的表达未见报道。本研究发现,夏季畜舍高温使Apaf-1和Caspase-9表达量升高。qRT-PCR和Western印迹结果显示,与对照组（正常舍温20℃）相比,短时热应激组（40～42℃,1 h/d, 7 d）和长时热应激组（40～42℃,1 h/d, 42 d）,Apaf-1和Caspase-9 mRNA和蛋白的相对表达量均显著升高。免疫组织化学研究发现,Apaf-1在猪睾丸组织中免疫反应阳性物定位于间质细胞、支持细胞和各个发育阶段生精细胞。热应激处理导致精母细胞和精子细胞Apaf-1表达量升高。在各实验猪睾丸组织中,Caspase-9定位于间质细胞、支持细胞和各个发育阶段生精细胞的胞质中。与对照组相比,热应激处理导致减数分裂以后的生精细胞和支持细胞Caspase-9表达量升高。上述结果表明,高温热应激促进Apaf-1和Caspase-9的表达,提示Apaf-1和Caspase-9表达的变化可能与猪舍高温导致的猪精液品质下降存在关联。     

孤儿受体TR3在小鼠睾丸中的定位和表达

本文采用原位杂交和免疫组织化学技术,观察孤儿受体ＴＲ３及其ｍＲＮＡ在小鼠睾丸中的表达及细胞定位。结果表明,在小鼠睾丸中有显著量的孤儿受体ＴＲ３ ｍＲＮＡ和蛋白表达,其表达量在不同曲细精管有明显的差异;孤儿受体ＴＲ３蛋白主要定位于生精细胞,其ｍＲＮＡ在生精细胞特异表达,主要在精原细胞和发育早期的初级精母细胞表达,提示孤儿受体ＴＲ３在小鼠曲细精管精子发生的早期阶段中起着调控作用。     

不同病理睾丸组织中雄激素受体和热休克蛋白90α表达的差异

目的检查和分析不同病理睾丸组织雄激素受体和热休克蛋白90α表达的差异.方法运用免疫组织化学二步法检查精子发生停滞、精原细胞瘤、前列腺癌去势和正常健康睾丸标本之雄激素受体和热休克蛋白90α的表达情况.结果正常睾丸组织和前列腺癌去势睾丸中雄激素受体在间质细胞、支持细胞和精原细胞的胞核表达,前者的表达强度高于后者(P<0.05);热休克蛋白90α主要在类肌细胞、间质细胞、支持细胞核及生精细胞的胞浆表达.精子发生阻滞的睾丸组织,雄激素受体主要在支持细胞的胞核和生精细胞的胞浆表达,热休克蛋白90α主要在支持细胞、类肌细胞表达;精原细胞瘤的睾丸组织,雄激素受体在肿瘤细胞的胞浆和胞核表达,热休克蛋白90α的表达强度在精原细胞瘤组织高于对照标本.结论雄激素受体核转运异常与精子发生阻滞有紧密关系;前列腺癌去势患者睾丸组织中,雄激素受体免疫反应强度减弱与睾丸衰老有关;精原细胞瘤患者睾丸标本,雄激素受体表达减弱,但热休克蛋白90α表达增强;提示雄激素受体和热休克蛋白90α的表达异常与精原细胞瘤的病理发生有关.     

原癌基因FOS蛋白、雌二醇及其受体在中国林蛙不同时期精巢中的表达

用免疫细胞化学方法检测了原癌基因FOS蛋白、17β-雌二醇(E2)和雌激素受体(ER)在中国林蛙生精周期中不同时期精巢内的表达定位。结果显示:在中国林蛙生精周期的Ⅰ—Ⅴ期,E2和ER在精原细胞、精母细胞、精子细胞、精子、支持细胞和间质细胞内均有表达。在不同时期的精巢中,E2和ER在生精细胞的定位具有一致性:在Ⅱ—Ⅲ期,精子细胞的E2和ER阳性表达最强;在Ⅲ期,精子中E2和ER阳性反应强度显著高于Ⅳ—Ⅴ期(P<0.01)。在生精周期的Ⅰ—Ⅴ期,支持细胞中,E2和ER表达强度经历由强减弱再增强的变化过程。在生精周期的Ⅲ期,间质细胞中E2和ER阳性反应强度高于其他各期。除精子外的生精细胞,支持细胞和间质细胞内均有FOS阳性反应,其表达强度呈现阶段性变化。     

SRG4在出生后小鼠睾丸及隐睾中的表达特性

研究小鼠生精新基因SRG4在出生后小鼠睾丸及手术隐睾中的表达特性, 为了解SRG4在精子发生中的作用奠定基础。取出生后1, 3, 12 w小鼠睾丸进行免疫组化检测, 观察SRG4蛋白在出生后小鼠不同发育阶段睾丸中的表达; 制备单侧手术隐睾模型, 取术后0~18 d 的隐睾组织进行半定量RT-PCR检测, 观察SRG4 mRNA在隐睾病变过程中的表达变化, 并对隐睾术后18 d 睾丸进行组织原位杂交分析。免疫组化分析结果表明, SRG4蛋白在出生1 w的小鼠睾丸中几乎检测不到, 在出生3 w的小鼠睾丸中有明显表达, 在出生12 w的小鼠中大量表达, 主要分布在精母细胞和圆形精子细胞胞浆及胞膜, 呈不均匀分布。半定量RT-PCR结果发现, SRG4 mRNA在小鼠隐睾术后0~6 d表达没有明显下调, 9 d 开始表达下调, 第18 d表达最低。组织原位杂交结果表明, 术后18 d隐睾睾丸生殖细胞大量凋亡, 精曲小管中仅见到个别的SRG4阳性信号, 而对照则不受影响。上述结果说明, SRG4蛋白表达受小鼠生长发育调控; 隐睾模型中, 随着生殖细胞的大量凋亡, SRG4基因表达下调, 提示SRG4基因可作为一个精子发生特定阶段的分子标记用以研究精子发生过程。     

LIM结构域蛋白KyoT在成年小鼠睾丸的表达

报道了KyoT在成年小鼠体内的表达,以便进一步研究KyoT在体内的功能。为研究KyoT mRNA及蛋白质水平的表达,采用Northern印迹、RT－PCR、免疫组织化学SABC和原位杂交方法。睾丸中两种KyoT的mRNA水平均很高,睾丸间质细胞的免疫化学反应阳性,阳性物质分布于细胞质内,细胞核呈阴性反应。同样,KyoT的mRNA在睾丸间质细胞杂交信号呈阳性反应,阳性物亦分布于细胞质内,细胞核呈阴性反应。生精细胞及对照组均为阴性。上述结果提示睾丸中有KyoT的表达,且特异性分布于睾丸间质细胞。     

大鼠睾丸雄激素受体表达的增龄变化

应用免疫细胞化学及图像分析等方法,对出生到生后25月龄各发育阶段SD大鼠睾丸内雄激素受体(AR)的表达变化进行了系统的研究。发现(1)睾丸间质细胞：从出生到生后3周龄,AR阳性表达强度较弱;到生后1月龄,AR阳性表达强度显著增强,并达到峰值;在生后2月龄,AR阳性表达强度显著减弱,此后AR阳性表达又呈增强趋势。(2)肌样细胞：从出生到生后2周龄,AR阳性表达强度较弱;到生后3周龄,AR阳性表达强度显著增强,并一直维持到生后2月龄;从生后3月龄,AR阳性表达强度呈减弱趋势,到生后25月龄达到最低水平。(3)血管内皮细胞：从生后3周龄到生后2月龄AR阳性表达较强;生后3月龄,AR阳性表达强度明显减弱;生后25月龄,AR阳性表达强度与生后3月龄相比变化不明显。(4)支持细胞：在生后1月龄出现AR阳性表达,到性成熟后,支持细胞AR阳性表达随生精周期变化而变化,在生后25月龄未见AR阳性表达的支持细胞。(5)生精细胞：出生组,前精原细胞内有AR阳性表达;生后2周龄,精子细胞开始出现AR阳性表达;生后1月龄,精原细胞开始出现AR阳性表达;生后2月龄出现阳性表达的精子,生后25月龄未见阳性表达的生精细胞。     

Beta-nerve growth factor influences the expression of androgen-binding protein messenger ribonucleic acid in the rat testis.

The effect of infusion of nerve growth factor (NGF) into the rat testis on the expression of androgen-binding protein (ABP) mRNA was studied. A major 1.7-kb and a minor 3.7-kb ABP mRNA were present at all stages of the seminiferous epithelium with maximal levels at stages VIII-XI and the lowest levels at stages IV-VI. Infusion of 15 ng/h of NGF with a mini-osmotic pump for 14 days resulted in a 2-fold increase of ABP mRNA as revealed by Northern blots, whereas the mRNA level of another Sertoli cell protein, urokinase-type plasminogen activator, remained unchanged. Image analysis of autoradiograms obtained by in situ hybridization of sections from treated testes showed a similar increase in APB mRNA compared to noninfused or PBS-infused testes. However, at the cellular level the labeling intensity for ABP mRNA over Sertoli cells of different stages of the seminiferous epithelium was the same in NGF-infused and control testes. This suggests that the increase of ABP mRNA in NGF-infused testes was caused by prolongation of stages VII-VIII with maximal ABP mRNA expression; the suggestion is supported by an increase of 30 percent in frequency of these stages in histological sections from NGF-infused testes.     

MTNR1a和MTNR1b在牦牛不同组织中的表达及其在睾丸中的定位

褪黑素对调节季节性繁殖哺乳动物的生殖具有重要调节作用。其受体MTNR1a（Melatonin receptor 1a,褪黑素受体1a）主要参与昼夜节律和生殖调控,MTNR1b（Melatonin receptor 1b,褪黑素受体1b）与多种疾病发生密切相关。为了探讨褪黑素受体基因的生物学功能,本实验对牦牛不同组织中MTNR1a、MTNR1b基因的表达与定位情况进行了研究。采用qRT-PCR (Quantitative Real-Time PCR, qRT-PCR) 检测成年雄性牦牛各组织及不同发育阶段（30日龄,2岁、4岁、6岁和8岁龄）牦牛睾丸组织中MTNR1a、MTNR1b mRNA的表达规律,并运用免疫组化技术对不同年龄牦牛睾丸中MTNR1a、MTNR1b蛋白进行了定位研究。结果发现,MTNR1a mRNA在松果体组织中表达量最高,肺脏、肌肉和睾丸次之;随着年龄增加,MTNR1a mRNA在睾丸中的表达量逐渐升高,到4岁后表达量趋于平稳;MTNR1a蛋白在不同发育阶段牦牛睾丸组织中均有表达,圆形精子呈现较强的免疫阳性,其次为初级精母细胞;MTNR1b mRNA在松果体表达量最高（P<0.05）,肾脏、肝脏和下丘脑次之;在不同年龄牦牛睾丸中MTNR1b mRNA均有表达,且随着年龄的增加表达量逐渐增加,在8岁时表达量最高;MTNR1b蛋白主要定位在圆形精子细胞中。MTNR1a、MTNR1b基因在牦牛不同组织及不同发育阶段睾丸中的广泛表达,揭示了其在雄性牦牛生殖等生理过程中的重要作用。     

PKC-α和PKC-δ在不同发育阶段小鼠睾丸中的差异性表达

蛋白激酶Ｃ(ＰＫＣ)作为一类重要的蛋白激酶 ,通过对底物蛋白的Ｓｅｒ Ｔｈｒ残基的磷酸化 ,参与细胞的短期反应与长期反应的调节 ,具有介导细胞生长和增殖 ,调节核基因的表达 ,影响细胞周期等生理作用 ,从而参与调控多种细胞系 ,如ＮＩＨ3Ｔ3细胞、造血干细胞等细胞系的增殖与分化[1,2 ] .在精子形成这样一个独特的细胞分化过程中 ,ＰＫＣ的生理功能仍未十分明确 .睾丸生殖细胞的增殖与分化 (精子发生 )是一个独特复杂的细胞分化过程 ,主要分为 3个阶段 :Ａ型精原细胞增殖和Ｂ型精原细胞分化为初级精母细胞 ;初级精母细胞通过减数分裂形成…     

Expression and localization of nerve growth factor (NGF) in the testis of alpaca (llama pacos)

During alpaca testis development and spermatogenesis, nerve growth factor (NGF) may play an important role. The main aim of this study was to determine the expression and localization of NGF in the alpaca testis, and to discuss the important role of NGF in alpaca reproductive characteristics. Immunohistochemical staining technique and real-time PCR were used. The expression of NGF in the same cells one-month old (newborn) alpacas 12-month, and 24-month old alpacas showed significant differences (p < 0.05); 12- and 24-month old alpacas showed no significant differences (p > 0.05); NGF at different cell stages showed no significant differences (p > 0.05). It suggests that NGF may be involved in the regulation of spermatogenesis, which provides direct evidence for NGF action in the alpaca testis during postnatal development and spermatogenesis.     

bFGF、NGF、EGF及其受体在人胚神经管早期发育中的表达

研究bFGF、NGF、EGF及其受体在人胚神经管早期发育中的表达。方法 应用免疫组织化学方法和图像分析。结果显示bFGF和NGF的表达时序不同,bFGF阳性细胞出现较早,在所检测在各个发育阶段均呈阳性表达,而NGF出现较晚,随着胚龄增加,免疫阳性着色逐渐增强,bFGF分布较NGF广泛,而EGF在所检测的各个发育阶段均呈阴性。flg、TrkA、EGFR表达时序和分布相似,三者在所检测的各个发育阶段均阳性。结果表明NGF和bFGF均通过其特异性受体介导,在胚胎神经管形成和分化的不同阶段发挥着重作用,EGF及其受体的作用有待进一步研究。     

Cloning, characterization and primary function study of a novel gene, Cymg1, related to family 2 cystatins

Cystatins are cysteine proteinase inhibitors. We found two expression sequence tags (ESTs), CA463109 and AV042522, from a mouse testis library using Digital differential display (DDD). By electrical hybridization, a novel gene, Cymg1 (GenBank accession No. AY600990), which has a full length of 0.78kb, and contains four exons and three introns, was cloned from a mouse testis cDNA library. The gene is located in the 2G3 area of chromosome 2. The full cDNA encompasses the entire open reading frame, encoding 141 amino acid residues. The protein has a cysteine protease inhibitor domain that is related to the family 2 cystatins but lacks critical consensus sites important for cysteine protease inhibition. These characteristics are seen in the CRES subfamily, which are related to the family 2 cystatins and are expressed specifically in the male reproductive tract. CYMG1 has a 44% (48/108) identity with mouse CRES and 30% (42/140) identity with mouse cystatin C. Northern blot analysis showed that the Cymg1 is specifically expressed in adult mouse testes. Cell location studies showed that the GFP-tagged CYMG1 protein was localized in the cytoplasm of HeLa cells. Immunohistochemistry revealed that the CYMG1 protein was expressed in mouse testes spermatogonium, spermatocytes, round spermatids, elongating spermatids and spermatozoa. RT-PCR results also showed that Cymg1 was expressed in mouse testes and spermatogonium. The Cymg1 expression level varied in different developmental stages: it was low 1 week postpartum, steadily increased 2 to 5 weeks postpartum, and was highest 7 weeks postpartum. The expression level at 5 weeks postpartum was maintained during 13 to 57 weeks postpartum. The Cymg1 expression level in the testes over different developmental stages correlates with the mouse spermatogenesis and sexual maturation process. All these indicate that Cymg1 might play an important role in mouse spermatogenesis and sexual maturation.     

Regulation of GDF9 and CDKN1B expression in Tibetan sheep testes during different stages of maturity

Normal spermatogenesis is heavily dependent on the balance of germ cell proliferation, differentiation and apoptosis. Growth differentiation factor 9 (GDF9) and cyclin-dependent kinase inhibitor 1 B (CDKN1B) are strongly associated with cell cycle transition from G0/G1 to S and G2/M phase and hence regulating the growth and development of testicular germ cells and somatic cells. The current study was aimed at seeking out scientific evidence to determine if GDF9 and CDKN1B gene expression functions in the development of Tibetan sheep testes. To this end, developmental testes were derived from three-month-old (pre-puberty), one-year-old (sexual maturity), and three-year-old (adult) Tibetan sheep and then the expression and localization patterns of GDF9 and CDKN1B in these testes were evaluated using quantitative real-time PCR (qRT-PCR), Western blot and immunofluorescence. qRT-PCR and Western blot results showed that GDF9 and CDKN1B were detected in the testes throughout the different developmental stages. The abundance of GDF9 mRNA and protein in the testes of one- and three-year-old Tibetan sheep were higher than that in the testes of three-month-old Tibetan sheep; the mRNA and protein abundance of the CDKN1B gene in three-month-old Tibetan sheep testes were higher than that in the testes of the one-and three-year-old sheep. Moreover, immunofluorescence results suggested that the GDF9 protein was expressed in spermatogonia and Leydig cells, and that the CDKN1B protein was localized mainly in Leydig cells with some in the seminiferous epithelium throughout developmental stages. This indicated a novel role of the GDF9 and CDKN1B genes in Leydig cell development over and above their known roles in germ cell development. These findings have significant implications for our understanding of the molecular mechanisms of GDF9 and CDKN1B genes in Tibetan sheep spermatogenesis.     

Cloning,Characterization and Primary Function Study of a Novel Gene,Cymg1,Related to Family 2 Cystatins

Cystatins are cysteine proteinase inhibitors,We found two expression sequence tags (ESTs),CA463109 and AV042522,from a mouse testis library using Digital differential display (DDD).By electricalhybridization,a novel gene,Cymgl(GenBank accession No.AY600990),which has a full length of 0.78 kb,and contains four exons and three introns,was cloned from a mouse testis eDNA library.The gene is locatedin the 2G3 area of chromosome 2.The full eDNA encompasses the entire open reading frame,encoding 141amino acid residues.The protein has a cysteine protease inhibitor domain that is related to the family 2cystatins but lacks critical consensus sites important for cysteine protease inhibition.These characteristicsare seen in the CRES subfamily,which are related to the family 2 cystatins and are expressed specifically inthe male reproductive tract.CYMG1 has a 44%(48/108)identity with mouse CRES and 30%(42/140)identity with mouse cystatin C.Northern blot analysis showed that the Cymgl is specifically expressed inadult mouse testes.Cell location studies showed that the GFP-tagged CYMG 1 protein was localized in thecytoplasm of HeLa cells,lmmunohistochemistry revealed that the CYMG1 protein was expressed in mousetestes spermatogonium,spermatocytes,round spermatids,elongating spermatids and spermatozoa.RT-PCRresults also showed that Cymgl was expressed in mouse testes and spermatogonium.The Cymgl expressionlevel varied in different developmental stages:it was low 1 week postpartum,steadily increased 2 to 5 weekspostpartum,and was highest 7 weeks postpartum.The expression level at 5 weeks postpartum was main-tained during 13 to 57 weeks postpartum.The Cymgl expression level in the testes over different develop-mental stages correlates with the mouse spermatogenesis and sexual maturation process.All these indicatethat Cymgl might play an important role in mouse spermatogenesis and sexual maturation. Cystatins are cysteine proteinase inhibitors,We found two expression sequence tags(ESTs),CA463109 and AV042522,from a mouse testis library using Digital differential display (DDD).By electricalhybridization,a novel gene,Cymgl(GenBank accession No.AY600990),which has a full length of 0.78 kb,and contains four exons and three introns,was cloned from a mouse testis eDNA library.The gene is locatedin the 2G3 area of chromosome 2.The full eDNA encompasses the entire open reading frame,encoding 141amino acid residues.The protein has a cysteine protease inhibitor domain that is related to the family 2cystatins but lacks critical consensus sites important for cysteine protease inhibition.These characteristicsare seen in the CRES subfamily,which are related to the family 2 cystatins and are expressed specifically inthe male reproductive tract.CYMG1 has a 44%(48/108)identity with mouse CRES and 30%(42/140)identity with mouse cystatin C.Northern blot analysis showed that the Cymgl is specifically expressed inadult mouse testes.Cell location studies showed that the GFP-tagged CYMG 1 protein was localized in thecytoplasm of HeLa cells,lmmunohistochemistry revealed that the CYMG1 protein was expressed in mousetestes spermatogonium,spermatocytes,round spermatids,elongating spermatids and spermatozoa.RT-PCRresults also showed that Cymgl was expressed in mouse testes and spermatogonium.The Cymgl expressionlevel varied in different developmental stages:it was low 1 week postpartum,steadily increased 2 to 5 weekspostpartum,and was highest 7 weeks postpartum.The expression level at 5 weeks postpartum was main-tained during 13 to 57 weeks postpartum.The Cymgl expression level in the testes over different develop-mental stages correlates with the mouse spermatogenesis and sexual maturation process.All these indicatethat Cymgl might play an important role in mouse spermatogenesis and sexual maturation.     

MYB基因在玉米雌穗发育中差异表达的研究

目的:研究MYB基因在玉米雌穗不同发育阶段的表达情况,为探讨其生物学功能提供相关线索。方法:用芯片杂交的方法检测玉米雌穗早期发育过程中差异表达的MYB基因,定量PCR验证差异基因的表达情况,原位杂交分析差异基因的组织器官表达。结果:一个MYB基因在雌穗发育到小花分化期时上调表达(芯片分析其表达差异倍数为1.8)。其表达的差异性得到了定量PCR的验证(定量PCR分析其差异表达倍数为4.3)。原位杂交分析发现该基因主要表达于小穗的生长锥顶部和小花雌雄蕊原基部位。结论:MYB基因对玉米雌穗早期发育起到一定作用。