789 resultados para César, Cayo Julio, 100-44 a. C.
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Heteropolyacids (HPAs) supported on the activated carbon (SiW12/C and PW12/C) have been used to study the formation of methyl tert-butyl ether (MTBE). Compared to the conventional commercial catalysts, Amberlyst-15 resin and HZSM-5, HPAs supported catalysts have been proved to have much higher catalytic activity under lower temperature, especially selectivity to MTBE is up to 100%. It may be due to the high acid strength of HPAs as well as the specialty of heteropolyanion.
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To improve the mechanics properties of polyurethane materials at a high or low temperature, a hydroxy compound N-100 of HDI was synthesized, The structure analysis and characterization were made by NMR (H-1, C-13, H-1-H-1 COSY, C-13-H-1 COSY), In addition, quantitative description of the network was made on the basis of some ideal assumptions, 1D and 2D NMR can differentiate four sorts of carbonyl groups and establish the connections of all carbon and hydrogen atoms of mixed structures that originated from five different substitutions, Besides, the alkene and isocyanate, urea, biuret and trimerized isocyanuric groups were also detected, Therefore, the structure of N-100 was suggested be a polyisocyanate with complicated network which contained nitrogen atom as cross-linkage, isocyanate and alkene as end groups, The consistence of calculated values with tested values of isocyanate content, mean function degree and mean molecular weight demonstrated the correct of structure characterization and the validity of network description.
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The conformational transition of horse heart cytochrome c induced by bromopyrogal red (BPR) in very low concentration has been firstly investigated by dynamic spectroelectrochemical technique, both at the BPR adsorbed platinum gauze electrode and at a bare platinum gauze electrode in a solution containing BPR. The effect of BPR on the structure of cytochrome c was studied by UV-visible and Fourier transform IR spectroscopy. The unfolded cytochrome c behaves simply as an electron transfer protein with a formal potential of -142 mV vs. a normal hydrogen electrode. The difference between the formal potentials of the native and unfolded cytochrome c is coupled to a difference in conformational energy of the two states of about 40 kJ mol(-1), which agrees well with the result reported. The stability and slow refolding of the unfolded cytochrome c are discussed.
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本文利用顺磁稀土离子的诱导化学位移变化的性质,研究了多官能团配体谷胱甘肽(GSH)与稀土的配位作用.在水溶液中GSH通过分子两端的羧基负离子与稀土形成遥爪配位结构.谷氨酸端和甘氨酸端羧基与Eu~(3+)的配位稳定常数分别为12.5±0.1L/mol和100.0±0.5L/mol.从~(13)C学位移的pH变化曲线求得谷氨酸端和甘氨酸端羧基解离的pK_a分别为2.20±0.02和3.50±0.04.对Dy~(3+)、Ho~(3+)、Er~(3+)、Tm~(3+)和 Yb~(3+)作用下,GSH的~(13)C移数据分析表明,配体与这些离子形成同构的配合物,分子两端羧基均可能以双齿形式与稀土配位.
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The condensation and sulfonation of furfuryl alcohol (FA) and FA with tris (2-hydroxyethyl) isocyanurate (THEIC) and the crosslinking product structures were studied by means of solid-state C-13 NMR. The reaction of formalin with FA linear oligomer terminated by 2-methyl furan took place in the presence of the phase transfer catalyst (C4H9)4N+I-. The reaction of the terminated oligomer with a large amount of sulfuric acid as well as the former reaction was examined. The effects of some main reaction conditions on the crosslinking condensation and sulfonation were also discussed.
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用固体~(13)C NMR研究了呋喃醇(FA)和FA三-(2-羟乙基)-异氰酸尿酯(THEIC)缩聚磺化反应及其产物结构,考察了2-甲基呋喃封端的FA型齐聚物与甲醛水溶液在相转移催化剂(C_4H_9)_4N~+I~-和与大量硫酸作用下的反应特点,探讨了主要参数对反应的影响,阐明了缩聚交联磺化反应的规律,确定了产物的结构。
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C12H12I2Te4, M(r) = 920.44, monoclinic, P2(1)/n, a = 10.942 (2), b = 14.924 (2), c = 11.415 (2) angstrom, beta = 104.32 (1)-degrees, V = 1806.0 (5) angstrom 3, Z = 4, D(x) = 3.38 g cm-3, lambda(Mo K-alpha) = 0.71069 angstrom, mu = 100.7 cm-1, F(000) = 1592, T = 294 K, R = 0.033 for 1828 observed reflections. One of the Te atoms is bonded to the two I atoms, which are on either side of the molecular plane. The Te-I distances are 2.963 (1) and 2.961 (1) angstrom, which means oxidation at the Te atom instead of at the C = C bonds.
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The precociously sexual maturation in large yellow crocker Pseudosciaena crocea has become a serious problem. In an attempt to solve this problem, the production of sterile triploids could be an effective strategy. In this study, triploid P. crocea was obtained by subjecting fertilized eggs to pressure shock. Flow-cytometry analysis was used to assess ploidy level. In terms of triploid rate and hatching rate, the optimal conditions of pressure shock for triploidy induction in P. crocea were 7500 psi for 3 min shock at 3 min after fertilization at 20 degrees C. With the application of these parameters, 100% triploid fish were produced. During the first rearing year, triploid P. crocea had a similar growth performance compared with its diploid counterpart before the age of 8 months and showed a significant advantage at the age of 10 and 12 months in body weight and body length (P < 0.05). At the age of 12 months, the carcass weight of triploids was markedly higher than that of diploid control, and gonadal somatic index was significantly lower than that of their diploid control. During the first rearing year, survival in triploid group was 76.44%, inferior to its diploid control (83.21%).
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Lectin is regarded as a potential molecule involved in immune recognition and phagocytosis through opsonization in crustacean. Knowledge on lectin at molecular level would help us to understand its regulation mechanism in crustacean immune system. A novel C-type lectin gene (Fclectin) was cloned from hemocytes of Chinese shrimp Fenneropenaeus chinensis by 3' and 5' rapid amplification of cDNA ends (RACE) PCR. The full-length cDNA consists of 1482 bp with an 861 bp open reading frame, encoding 287 amino acids. The deduced amino acid sequence contains a putative signal peptide of 19 amino acids. It also contains two carbohydrate recognition domains/C-type lectin-like domains (CRD1 and CRD2), which share 78% identity with each other. CRD1 and CRD2 showed 34% and 30% identity with that of mannose-binding lectin from Japanese lamprey (Lethenteron japonicum), respectively. Both CRD1 and CRD2 of Fclectin have I I amino acids residues, which are relatively invariant in animals' C-type lectin CRDs. Five residues at Ca2+ binding site I are conserved in Fclectin. The potential Ca2+/carbohydrate-binding (site 2) motif QPD, E, NP (Gln-Pro-Asp, Glu, Asn-Pro) presented in the two CRDs of Fclectin may support its ability to bind galactose-type sugars. It could be deduced that Fclectin is a member of C-type lectin superfamily. Transcripts of Fclectin were found only in hemocytes by Northern blotting and RNA in situ hybridization. The variation of mRNA transcription level in hemocytes during artificial infection with bacteria and white spot syndrome virus (WSSV) was quantitated by capillary electrophoresis after RT-PCR. An exploration of mRNA expression variation after LPS stimulation was carried out in primarily cultured hemocytes in vitro. Expression profiles of Fclectin gene were greatly modified after bacteria, LPS or WSSV challenge. The above-stated data can provide us clues to understand the probable role of C-type lectin in innate immunity of shrimp and would be helpful to shrimp disease control. (c) 2006 Elsevier Ltd. All rights reserved.
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C-type lectin is a family of Ca2+ dependent carbohydrate-recognition proteins which play crucial roles in the innate immunity of invertebrates by mediating the recognition of host cells to pathogens and clearing microinvaders as a pattern recognition protein (PRP). The cDNA of Zhikong scallop Chlamys farreri C-type lectin (designated CFLec-1) was cloned by expressed sequence tag (EST) and RACE techniques. The full-length cDNA of CFLec-1 was 1785 bp, consisting of a 5'-terminal untranslated region (UTR) of 66 bp and an unusually long 3' UTR of 1040 bp with seven polyadenylation signal sequences AATAAA and a poly(A) tail. The CFLec-1 cDNA encoded a polypeptide of 221 amino acids with a putative signal peptide of 15 amino acid residues and a mature protein of 206 amino acids. Analysis of the protein domain features indicated a typical long-form carbohydrate-recognition domain (CRD) of 130 residues in the CFLec-1 deduced amino acid sequence. The expression pattern of CFLec-1 transcripts in healthy and bacterial challenged scallops was studied by semi-quantitative RT-PCR. mRNA transcripts of CFLec-1 could be mainly detected in the tissues of haemocytes, gill, gonad and mantle of unchallenged scallops, whereas the expression of CFLec-1 transcripts was increased in all the tested tissues after heat-killed Vibrio anguillarum challenge. The temporal expression of CFLec-1 mRNA in haemolymph challenged by Micrococcus luteus and V anguillarum was both up-regulated and reached the maximum level at 8 and 16 It post stimulation, respectively, and then dropped back to the original level. In order to investigate its immune functions, CFLec- I was recombined and expressed in Escherichia coli BL21(DE3)-pLysS as a fusion protein with thioredoxin. The recombinant CFLec-1 agglutinated bacteria E. coli JM109 in vitro, and the agglutination was Ca2+ dependent which could be inhibited by EDTA. But it did not agglutinate M. luteus, Candida lipolytica and animal erythrocytes including rabbit, rat, mouse, chicken, human group A, human group B, human group O. Meanwhile, the recombinant CFLec-1 could inhibit the growth of both E. coli JM 109 and M. luteus, but no inhibition activity against V anguillarum. These result indicated that CFLec-1 was a constitutive and inducible PRP which was involved in the reorganization and clearance of invaders in scallop. (c) 2006 Elsevier Ltd. All rights reserved.
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Large yellow croaker, Pseudosciaena crocea, exhibit sexually dimorphic growth, with females growing faster and reaching larger adult sizes than males. Thus, development of techniques for preferentially producing females is necessary to optimize production of these species. We have established a protocol to produce all-female croaker P. crocea through induction of meiotic gynogenesis with homologous sperm. The first set of experiments investigated the ultra-violet (UV) irradiation on sperm motility and duration of sperm activity to determine the optimal UV dosage for genetic inactivation of sperm, yet retaining adequate motility for activation of eggs. Milt from several males was diluted 1: 100 with Ringer's solution and UV irradiated with doses ranging from 0-150 J cm (-2). The results indicated that motility and duration of activity generally decreased with increased UV doses. At UV doses greater than 105 J cm(-2), after fertilization, motility was < 10% and fertilization rates were significantly lower. Highest hatching rate was obtained at 75 J cm -2. A second set of experiments was carried out to determine appropriate conditions of cold shock for retention of the 2nd polar body in P. crocea eggs after fertilization with UV-inactivated sperm by altering the timing, temperature and duration of shock. At 208 degrees C, shock applied at 3 min after fertilization resulted in higher survival rate of larvae at 6 h after hatching. Results of different combinations of three shock temperatures ( 28 degrees C, 38 degrees C or 48 degrees C) and five shock durations ( 4 min, 8 min, 12 min, 16 min or 20 min) at 3 min after fertilization demonstrated that shocks of 12 min gave highest production of diploid gynogens. Statistical analysis revealed that maximum production of diploid gynogens (44.55 +/- 2.99%) were obtained at 38 degrees C. The results of this study indicate that the use of UV-irradiated homologous sperm for activation of P. crocea eggs and cold shock for polar body retention is an effective method for producing gynogenetic offspring.
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Pure C-phycocyanin was prepared from Spirulina platensis using one-step anion-exchange chromatography. The C-PC obtained was with an absorption maximum at 620 nm and a fluorescence emission maximum at 640 nm when excited by 580 nm. SPDP is an excellent heterobifunctional crosslinker for thiolating amines. Different molar ratios of SPDP have remarkable influence on the absorption and fluorescence spectra of C-phycocyanin. The absorption maximum and fluorescence emission maximum both decreased and blue-shifted from 640 run to 630 nm as the molar ratios of SPDP increased. It was found that the molar ratios of SPDP to C-phycocyanin was not more than 100 was appropriate to being conjugated with other biomolecules from the absorption and fluorescence spectra of C-phycocyanin.
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海洋生物具有产生丰富多样的次生代谢产物的能力,其中红藻门松节藻科海藻卤代次生代谢产物以其结构新颖、生物活性独特引起了天然产物化学家的重视。 本论文对海洋红藻多管藻和松节藻进行了化学成分研究,综合利用各种色谱学方法 (硅胶柱层析、反相硅胶柱层析、凝胶Sephadex LH-20柱层析、半制备高效液相色谱以及重结晶等) 和现代波谱学技术 (IR、UV、EI-MS、FAB-MS、HR-ESI-MS、CD、1H-NMR、13C-NMR、DEPT、1H-1H COSY、HSQCHMBC),共分离鉴定了100个化合物,发现25个新化合物。 从多管藻中分离鉴定38个化合物 (24个溴酚化合物),其中7个新化合物 (均为溴酚化合物),包括1个菲并呋喃结构溴酚 (P1), 2个二氢菲结构溴酚 (P2, P3),1个含 5,7-dihydrodibenzo[c,e]oxepine 结构溴酚 (P4)和3个简单溴酚 (P5, P6, P7)。P1 (urceolatin) 属首例报道的具有菲并呋喃结构的天然产物,从该种中分离的化合物P12 和 P13 可能是其生源合成的前体。P2和P3为第二例报道的具有二氢菲结构的溴酚化合物。 从松节藻中分离并鉴定了62 个化合物,其中18 个为溴酚类新化合物,44 个为已知化合物。化合物具有多变的取代基团,包括2 个脲基吡咯烷酮溴酚化合物 (R1, R2), 4 个γ-脲基丁酸溴酚化合物 (R3-R6),5 个酰胺溴酚化合物 (R7, R8, R9, R13, R14),1 个溴酚砜化合物 (R12), 1 个Xanthene 溴酚化合物 (R10)和5 个简单溴酚化合物 (R11, R15, R16, R17, R18)。R1、R2 是首例报道的含有脲基吡咯烷酮片段的天然产物,R10 为首次报道的溴代Xanthene 类天然产物。 对分离到的化合物进行了清除DPPH 和ABTS两种自由基活性的筛选。结果发现溴酚类天然产物具有显著的DPPH自由基清除活性,其中R3 的IC50 仅为3.3 μM, 其活性强度约为阳性对照BHT (IC50 为82.1 μM) 的24倍。另外,溴酚类天然产物对ABTS自由基有较强的清除活性,R2 的TEAC(Trolox efficency activity capacity)值为5.2 mM,约为阳性对照 (ascorbic acid, 1.02 mM) 的 5 倍。初步的构效关系研究发现,稠环分子、多羟基和邻位甲氧基等结构特点能有效增强DPPH 自由基清除活性;特殊取代基如脲基、吡咯烷酮等含有氮原子的基团,能有效增强ABTS 自由基清除活性,多羟基、溴代等结构特点也使其活性有所增强。 本研究结果丰富了海藻卤代化合物的结构类型,为多管藻和松节藻的合理利用提供了一定的科学依据。
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本研究应用显带技术和荧光原位杂交(Fluorescence in situ hybridization,FISH)技术,鉴定了牡蛎的染色体;应用FISH方法定位了一系列的重复序列和大分子的P1克隆DNA制备了染色体特异性探针。应用FISH特异性探针成功地鉴定了长牡蛎的三体10。结果如下:1.分析了G带和C在美洲牡蛎染色体上的分布。G带在每一条染色体上的带型不同,某些染色体间(如第1对和第4对染色体,第7对和第9对染色体)的带型差别不是很明显。G带型容易受染色体收缩程度的影响。C型重复性较好,染色体带型较清楚,分布在染色体的端粒区域和着丝粒区域。G带和C带型能够用来鉴定牡蛎的染色体,但是重复性低和带型差异不显著,并不适合常规的染色体鉴定。2.早期胚胎和担轮幼虫制备的染色体适合于FISH分析。染色体制备方法重复性好,可适用于其它贝类的染色体制备。3.研究了重复序列基因--rDNA定位:1)18S-5.8S rDNA研究的五种巨蛎属Crassostrea蛎均只有一个位 点。太平洋种(C.gigas,C. ariakensis和C. plicatula)中,杂交信号位于最短的染色体一第10对染色体长臂的端粒区域,在大西洋种(C. virginica和C. rhizophorae)中,同一序列定位在第2对染色体短臂的端粒区域。2)18S-28S rDNA两种蛤中有两个位点。rDNA针定位在侏儒蛤(Mulinis Lateralis)的第15对和第19对染色体的端粒区域,同一序列定位在硬壳蛤(Mercenaria mercenaria)的第10对染色体的长臂和第12对染色体短臂的端粒区域。信号强度在两对染色体之间有差异。 3)5s rDNA于美洲牡蛎的第5对染色体的短臂上靠近着丝粒区域和第6 对染色体的短臂的中间区域。信号强度在两对染色体之间没有显著差异。5S rDNA针可以作为鉴定和识别第5对和第6对染色体的特异性探针。4.研究了一些重复序列的定位1)两个短的重复序列1G8,1P2均产生很强的荧光信号分布在美洲牡蛎所有的染色体上。在低严谨条件下,这些序列均产生很强的信号散布在所有的染色体上。在高严谨条件下,信号强度大大减弱,但是信号仍散布在所有的染色体上。这些重复序列散布在美洲牡蛎的整个基因组中。2)高度重复序列Cgl70产生的信号分布在长牡蛎的7对染色体的着丝粒区域,没有发现间区信号。在第1对,第2对,第4对和第7对染色体上的荧光信号强且稳定。在第5对,第8对和第10对染色体上的信号相对弱且不稳定。在剩余的染色体上(第3对,第6对和第9对染色体)没有检测到荧光信号。结果表明此卫星序列是一个着丝粒卫星序列。在美洲牡蛎的染色体上没有检测到荧光信号,表明了这个着丝粒卫星序列在这两种牡蛎中的分布存在着显著的差异。3)脊椎动物端粒序列(TTAGGG)n的FISH信号局限在四种双壳贝类(美洲牡蛎,the mangrove oyster,硬壳蛤,侏儒蛤)所有染色体的端粒区域,没有发现间区信号的存在。研究结果与已报道的研究结果表明脊椎动物端粒序列或许存在于所有双壳贝类的染色体末端。双壳贝类是目前研究过的唯一含有脊椎动物端粒序列DNA无脊椎动物。4)研究了RAPD探针在美洲牡蛎染色体上的定位。大多数RAPD探针产生了多个信号散布在间期细胞核和所有的染色体上。引物OPX-03,OPX-04,OPX—06,OPG-02,OPM—04,OPM-11,0PS-02制备的探针在适宜的条件下产生特异性荧光 信号,分布在牡蛎的特定的染色体上。PCR特异性带产生的探针OPX—06—310和0PG-02—300产生了特异性的荧光信号:OPX—06—310产生的信号位于第5对染色体的短臂的近端粒区域,0PG—02—300探针定位到第3对染色体的短臂上。这两个探针是鉴定美洲牡蛎单条染色体的特异性探针。5.研究了大分子Pl克隆DNA(插入片断为80~100 kb)在美洲牡蛎染色体上的定位。Pl克隆DNA过切口平移方法标记digoxigenin—11-dUTP用作FISH的探针。Cot-1 DNA为竞争剂有效地抑制了Pl克隆序列中的重复序列产生的信号。杂交信号用fluorescein标记的anti—digoxigenin抗体来检测,用两层抗体rabbit-anti-sheep抗体和FITC anti—rabbit抗体来扩增信号。9个P1探针成功地定位在特定的染色体上。46—1探针杂交到第1对染色体的长臂靠近着丝粒区域;47-10探针定位到第2对染色体的长臂近端粒区域;Cvpl和48-13两探针定位到第3对染色体上:Cvpl位于短臂的端粒区域,48-13探针位于长臂的近着丝粒区域;48—10探针杂交到第4对染色体的长臂上;48-1探针杂交到第5对染色体长臂的近着丝粒区域;49-11探针位于第7对染色体长臂上;探针49-10和44-11位于第8对染色体长臂上。同时我们成功地将2个P1探针杂交到同一染色体分裂相中,进一步确定了Pl探针在美洲牡蛎染色体 上的定位。6.应用18S-28S rDNA针成功地鉴定出长牡蛎非整倍体中的三体10。经鉴定AF-35,AF-39和AF-3三体家系属于三体10家系。rDNA针分布在三条染色体上,即多出的一条染色体为染色体10。相应地在间期细胞核上有三个信号出现。AF-34和AF-36家系不属于三体10家系。rDNA针分布在两条染色体上,相应地在间期细胞核上有两个信号出现。FISH和染色体特异性探针为非整倍体的鉴定提供了一个快速准确可靠的方法和途径。
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优良的种质是产业发展的重要保证,品种更新和养殖技术的发展已经给世界农业带来了令人瞩目的成就,然而我国水产生物的育种工作刚处于起步阶段,而育种技术的研究则更是滞后。借鉴陆生生物中发展起来的相对成熟的研究方法,可以帮助加快海洋生物遗传育种相关研究的进度。本研究以我国北方海区重要的海洋经济动物-皱纹盘鲍为研究对象,从表型遗传、数量性状遗传等2个方面开展了皱纹盘鲍的遗传育种研究,同时从幼鲍培育密度与分选效应等方面研究了皱纹盘鲍的中间培育技术。 主要结果如下: 1. 皱纹盘鲍的贝壳颜色遗传、食物对贝壳颜色表现型的影响,贝壳颜色与生长速度间的关系 将贝壳颜色为橘红色(O表型)的突变型皱纹盘鲍与贝壳颜色为绿色(G表型)的野生型皱纹盘鲍进行了连续2代的交配实验。结果表明:皱纹盘鲍橘红色的贝壳颜色相对于绿色的贝壳颜色为隐性性状,皱纹盘鲍的贝壳颜色表型受单位点、2个等位基因遗传控制,其中基因型为oo的个体,贝壳颜色的表现型为橘红色(O表型),而基因型为GG或Go的个体,贝壳颜色的表现型为野生型(G表型)。 为探讨食物类型对不同基因型皱纹盘鲍贝壳颜色表现型的影响,对不同贝壳颜色表型的个体投喂不同种类的食物,结果表明,除遗传因素外,皱纹盘鲍的贝壳颜色表现型显著地受食物类型的调控。其中oo基因型的个体,在摄食底栖硅藻(Navicula sp.)和红藻时,贝壳颜色的表型为橘红色;而在摄食褐藻、绿藻和以海带粉为唯一海藻源的人工配合饵料时,贝壳颜色的表型为黄色。GG和Go基因型的个体,在摄食底栖硅藻、红藻时,贝壳颜色的表型为褐红色;在摄食褐藻、绿藻和以海带粉为唯一海藻源的人工配合饵料时,贝壳颜色的表型为绿色。该结果表明,相同基因型的皱纹盘鲍在摄食不同类型的食物时,贝壳表现型不同,即不同类型的食物可以导致2种基因型皱纹盘鲍的贝壳颜色表现型在一定范围内发生转换:oo基因型的个体,贝壳的颜色可以表现为橘红色或者黄色,不会出现野生型皱纹盘鲍的褐红色或绿色;而GG与Go基因型的个体,相应的贝壳颜色表型只能是褐红色或者绿色,不会出现oo基因型可能表现的橘红色或黄色。特定基因型的皱纹盘鲍,在摄食特定类型的食物时贝壳的相应部位可表现出特定的颜色。皱纹盘鲍的这种“食物-贝壳颜色”的相关性可作为一种形态标记,用于标识皱纹盘鲍的个体和群体,该标记技术可用于皱纹盘鲍的养殖技术和遗传学研究。 此外,选用了贝壳颜色遗传学实验中建立的贝壳颜色发生分离的家系为实验材料,以壳长为指标,分析比较了来自相同家系的O表型与G表型个体之间的生长速度。结果表明,在幼鲍发育至412天止的3-5个统计时段内,没有在同一家系来源的2种贝壳颜色表型个体之间检验到生长速度的显著差异。 2. 皱纹盘鲍不同选育群体及杂交群体的贝壳形态参数分析 在皱纹盘鲍的7个群体中(包括已经对生长速度为指标进行了多代人工选育的群体4个、野生群体之间直接杂交繁育的杂交F1群体3个),测量了4-6龄成体样本的壳长(L)、壳宽(W)、壳高(H)和壳重(Sw),并计算了L/(L+W+H)、W/(L+W+H)、H/(L+W+H)和Sw/(L×W×H)等4个壳形态学参数。用方差分析方法(MANOVAANOVA统计并比较了这些壳形态参数在皱纹盘鲍群体间的遗传变异。结果表明,4个壳形态参数在不同群体间变异系数分别为0.34、0.74、2.62和6.54,其中,H/(L+W+H)与Sw/(L×W×H)在各供试群体间均具有较高的多态性且差异达显著水平,表明这2个参数在不同群体间存在较高的遗传变异。由于在活体情况下无法测量壳重(Sw)性状,建议以参数H/(L+W+H)为指标对皱纹盘鲍贝壳形态(如壳型)等进行人工选择。 3. 皱纹盘鲍成体阶段生长性状的遗传参数估计 采用巢式设计,分析了成体阶段不同发育期皱纹盘鲍的壳长与生长速率的遗传力、不同发育期的壳长性状之间的遗传相关、以及不同发育期的生长速率之间的遗传相关,结果表明:(1)壳长遗传力在受精后第70 、130、320、320、380、490与550天的雄性组分估计值分别为0.161 ± 0.075、0.312 ± 0.131、0.326 ± 0.331、0.135 ± 0.228、0.153 ± 0.185和0.180 ± 0.106;雌亲组分估计分别为0.312 ± 0.172、0.699 ± 0.168、0.695 ± 0.168、0.977 ± 0.407、0.427 ± 0.195和0.449 ± 0.027。(2)生长速率遗传力在受精后第320~380天、490 ~ 550天,雄、雌组分估计值分别为0.080 ± 0.120(雄)、 0.210 ± 0.191(雌)以及0.299 ± 0.146(雄)、0.306± 0.148(雌)。雌亲组分的壳长遗传力和生长速率遗传力估计值较大且均达显著水平,表明皱纹盘鲍在成体阶段依然受母性效应的影响。成体阶段生长性状遗传力水平的估计对制定科学的皱纹盘鲍育种方案有指导意义。(3)雄亲组分估计的不同发育期(第390 ~ 550天)壳长间遗传相关为0.597 ~ 1.000,雌亲组分估计为0.589 ~ 1.177。由雄亲、雌亲组分估计,受精后第320~380天与第490 ~ 550天两个发育阶段生长速率间遗传相关均接近于0。雌亲组分估计不同发育期壳长间遗传相关均达显著水平(t0.05, d.f.=13 = 4.33 ~ 11.69,P<0.01),表明壳长性状早期选择有效,即在皱纹盘鲍早期阶段依据壳长性状对个体进行择优或去劣可在后期阶段获得壳长较大的个体。由于使用的雄亲数目少(8个父系半同胞),实验中以雄亲组分估计的遗传参数误差较大。 4. 皱纹盘鲍选育系间的群体杂交 进行了皱纹盘鲍4个人工选育系之间的完全双列杂交实验,以群体交配的方式共建立了16个组合;此外,以大连“98”选群与汕头“S”选群为亲本,以群体交配的方式建立了4个交配组合。对不同方向的杂交组合进行了中亲杂种优势、超亲杂种优势以及配合力等方面的评价。 (1)测量了4个选育群体(R、97、S和J)及其各杂交组合在受精后第9、20和30天时的壳长,统计分析了不同选育系间壳长性状的差异、评价了不同方向杂交组合的中亲与超亲杂种优势、以及配合力。结果如下: 选育系群体内交配繁育的4个组合,在受精后第9、20和30天的壳长均有显著差异,其中,97 97组合在早期发育各阶段均为最小,分别为0.462 ± 0.023mm、0.698 ± 0.057mm和1.476 ± 0.234mm;S S组合的3次测量值均为最大,分别为0.522 ± 0.023mm、0.824 ± 0.084mm和1.798 ± 0.229mm。 两个方向杂交组合与选育系亲本群体内交配组合的平均值和高亲值比较,得到如下结果:(A受精后第9天壳长表现正向中亲杂种优势的组合有6个、表现负向中亲杂种优势的组合6个,其中J 97组合的中亲优势率最高,为9.05%;R S组合最低,为-6.61%。正向高亲杂种优势组合有4个、负向高亲杂种优势组合有8个,其中S J组合的高亲优势率最高,为5.77%;R S组合最低,为-7.96%。(B)受精后第20天壳长表现正向中亲杂种优势的组合有7个、表现负向中亲杂种优势的组合5个,其中J 97组合的中亲优势率最高,为12.60%;J R组合最低,为-8.72%。正向高亲杂种优势组合有3个、负向高亲杂种优势组合有11个,其中J 97组合的高亲优势率最高,为12.20%;J R组合最低,为-12.67%。(C受精后第30天壳长表现正向中亲杂种优势的组合有7个、负向中亲杂种优势的组合5个,其中97 S组合的中亲优势率最高,为24.08%;S 97组合最低,为-12.69%。正向高亲杂种优势组合有6个、负向高亲杂种优势组合有6个,其中97 S组合的高亲优势率最高,为15.95%;S J组合最低,为-19.44%。上述结果表明,皱纹盘鲍不同选育系之间的交配组合,杂种优势率差异很大,因此,通过组配实验,将杂种优势率高的交配组合选择出来应用于生产,可望显著提高目标性状的产量。 对早期发育阶段各生长期壳长性状,亲本一般配合力(GCA)、各杂交组合间特殊配合力(SCA)以及正反交(REC效应值进行方差分析,结果表明:各亲本GCA差异显著,说明各选育群体存在显著的遗传差异,其中汕头选群“S”在测量的各个生长期均为正值且显著大于其它各亲本;特殊配合力(SCA)以及正反交(REC效应值较大在各杂交组合间存在显著差异,说明在早期生长发育阶段非加性遗传效应(显性和上位效应)占主导地位。综合各个生长期亲本GCA和杂交组特殊配合力(SCA)以及正反交(REC效应值,杂交组合97×S在早期生长阶段不仅有较高SCA值而且两个亲本也具有较大的GCA值,表明选育系97和S较适宜作为杂交亲本使用。 (2)大连“98”选群与汕头“S”选群进行2×2因子设计的群体杂交实验,比较了各交配组合早期存活相关性状如受精率、孵化率、变态率以及壳长性状,评价了两个方向杂交组合平均以及不同方向杂交组合的中亲杂种优势率。结果表明早期发育阶段各组合间的受精率无显著差异,而孵化率、变态率等两个杂交方向平均的中亲杂种优势率为5.49%与12.53%,高于壳长性状的优势率(0.936-1.534%)。方差分析结果表明不同方向的杂交组合在早期发育阶段存活相关性状以及壳长性状存在显著差异。孵化率、变态率性状,S×98的中亲杂种优势率分别为13.21%与21.10%,均高于98×S的-3.84%与3.85%;而第10和25d壳长性状,S×98的中亲杂种优势率为1.14%与-2.52%,低于98×S的1.93%与4.41%。 为进一步评价“98”选群与“S”选群不同交配组合在不同温度条件下的生长,进行了基因型与环境的互作研究。从“98”选群与“S”选群的4个交配组合中分别取5月龄幼鲍100头,各组合随机分成3组,每组1个重复,分别于12°C16°C 22°C度条件下进行培育,比较各交配组合基因型与温度对幼鲍生长的影响。不同温度条件下,各组合壳长生长的方差分析结果表明,基因型和温度都能够对幼鲍生长以及最终壳长产生极显著的影响(P < 0. 01),它们的交互作用也达到显著水平(P < 0.05)。杂交子代的幼鲍壳长在12°C16°C 22°C度条件下均表现出杂种优势,双向杂交的中亲杂种优势率分别为5.32%、5.55%和0.03%,表明低温条件(12°C,比高温条件(22°C下有更强的杂种优势。汕头“S”选群的早期孵化率、变态率、生长性状以及低温条件下幼鲍生长性状的单亲杂种优势率分别为16.64%、42.49%、3.42~5.79%和5.73~9.15%,单亲杂种优势率较大,表明可通过杂交手段,显著地改良汕头“S”选群在早期发育阶段的生长速度、存活率以及幼鲍期的生长性状。本研究的结果支持了Lerner(1954)杂种优势的基因与环境互作学说。 5. 皱纹盘鲍幼鲍的中间培育技术研究 (1)对南方越冬方式的评价 目前,每年的11月前后,将6-7月龄幼鲍运往南方的闽东、闽中、闽南沿海越冬,翌年4月至6月再运回到北方(大连、山东半岛)的养殖模式已经普遍应用于皱纹盘鲍的实际生产,为评价南方越冬的幼鲍培育方式,本研究分别以不同幼鲍材料在闽东三都海湾进行了越冬培育实验。 选择生产上壳长分别为18.37 ± 1.28 mm、15.89 ± 1.10 mm、14.55 ± 1.10 mm与10.59 ± 0.84 mm的幼鲍进行了为期6.5个月的越冬培育,实验结束时,存活率分别为95.56 ± 2.21%、90.55 ± 1.96%、83.97 ± 1.63%与63.30 ± 2.79%。回归分析表明,供试幼鲍在实验起始时的壳长与越冬阶段的存活率成正相关(P = 0.018 < 0.05)。该结果表明,提高幼鲍的规格可显著提高皱纹盘鲍的越冬成活率,因此对于实际生产而言,采取适当措施提高皱纹盘鲍越冬苗种的规格将大幅增加生产的收益,而采用生长速率快的品种、品系或提早采苗均可实现该目标。综合各规格组幼鲍,幼鲍在南方开放性水域进行越冬培育的平均存活率较高,可达到91.38±0.01%,从幼鲍南方越冬的存活曲线可以看出,幼鲍的死亡主要集中在从大连运至福建某地后的15天内,出现死亡高峰的原因可能是由于运输过程的胁迫。此外,2月及4月中下旬水温出现显著降低或回升时也有较明显的死亡出现。该部分结果,对皱纹盘鲍幼鲍的养成管理有指导意义,可以通过合理安排越冬时间、避开死亡的敏感期等措施减少苗种越冬阶段的死亡量。 以中国大连野生群体繁育的子一代为亲本(10♀,10♂),以群体交配的方式繁育F2代个体为实验材料,分别于南方海区以及北方室内升温水方式下进行生长、存活比较,结果表明南方越冬培育方式下,幼鲍壳长的日增长率为81.37-108.89 µm•day-1,与北方室内升温培育条件相比,壳长生长提高了1.08 ~ 1.68倍;而存活率无显著差异。皱纹盘鲍幼鲍南方越冬方式的优势主要体现在鲍鱼幼鲍的生长速度加快,同时节约养殖场的能耗 (2)幼鲍培育过程中的养殖密度与分选效应评价 以3种规格皱纹盘鲍幼鲍为材料比较幼鲍在4个培育密度以及分选或混养条件下壳长的平均日生长及特定生长率。在南方越冬培育方式下实验进行106天,多因素方差分析结果表明实验初始幼鲍的壳长以及培育密度对壳长的生长有显著影响,而且密度效应在不同幼鲍起始规格组中有不同表现;分选没有能够提高不同规格组的生长。本研究的结果对皱纹盘鲍幼鲍的越冬培育有一定的指导作用。
