鲤鱼(Cyprinus carpio L.)体重和体长QTL的定位

利用265个AFLP标记、127个微卫星分子标记、37个EST-SSR标记和16个RAPD标记(共445个标记)对大头鲤/荷包红鲤抗寒品系的F2代雌核发育群体44个个体进行基因型检测,构建鲤鱼(Cyprinus carpio L.)遗传连锁图谱;利用软件WinQTLCart2.5采用复合区间作图法对体重和体长两个性状进行了QTL定位分析。结果共检测到与两个与体重性状相关的QTL,分别定位到LG24连锁群(qBWh-24-1)和LG20连锁群(qBWh-20-1)上,可解释的表型变异分别为7.98%和20.05%;检测到两个与体长性状相关的QTL,分别位于LG2连锁群(qFS-2-1)和LG20连锁群(qFS-20-1),可解释的表型变异分别为5.69%和12.69%,4个QTL的加性效应均为负值。

Effect of Certain Toxicants on Gonadotropin-Induced Ovarian Non-Esterified Cholesterol Depletion and Steroidogenic Enzyme Stimulation of the Common Carp Cyprinus carpio in vitro

Isolated ovarian tissues from the common carp, Cyprinus carpio were incubated in vitro to obtain a discrete effect of four common toxicants of industrial origin, namely phenol, sulfide, mercuric chloride and cadmium chloride, on gonadotropin-induced alteration of nonesterified and esterified cholesterol and steroidogenic enzymes, △5-3β-HSD and 17β-HSD activity. Stage II ovarian tissue containing 30-40% mature oocytes were shown to be most responsive to gonadotropins in depleting only nonesterified cholesterol moiety and stimulating the activity of both. Safe doses of above mentioned toxicants when added separately to stage II ovarian tissue with oLH (1 μg/incubation) gonadotropin-induced depletion of nonesterified cholesterol and gonadotropin-induced stimulation of the activity of both enzymes was significantly inhibited. Esterified cholesterol remained almost unaltered. Findings clearly indicate the impairment of gonadotropin induced fish ovarian steroidogenesis by the four toxicants separately.

Effect of Mercuric Chloride and Cadmium Chloride on Gonadal Function and Its Regulation in SexuallyMature Common Carp Cyprinus carpio

Gonadal function in fish, CJprinus carpio was significantly affected by sublethal doses of mercuric chloride (HgCl2 ) and cadmium chloride (CdCl2 ) in chronic (45 days ) exposure.Parameters investigated were nonesterified (NE) and esterified (E) cholestcrol of ovary,liver and serum and ovarian 3β-Hydroxysteroid and 17β-Hydroxysteroid dehyrogenaseenzyme activity and serum and pituitary gonadotropin (GtH) levels. Both the pollutantswere able to reduce the hypothalamic extract (HE) or gonadotropin releasing hormone(GnRH) induced pituitary GtH release in vitro. Short term (96h) exposure of the fish tothe pollutants had no significant effect on the gonadal function. ln addition to thedeleterious effect of pollutants on the gonadal steroidogenesis and pituitary gonadotropin release, using [4-14C] cholesterol as a tracer it was found that for 45 days expeure, HgCl2'had an adverse effect on the transport of cholesterol from circulation to ovary.

Ontogeny of Immune Related Organs during Early Development of Carp (Cyprinus Carpio L.)

In this paper, ontogeny of immune-related organs during theearly development of carp was studied by histochemical technique-lcineBlue staining under acid conditions and PAS reaction(AB-PAS staining). Thekidney appeared one day before hatching, spleen, liver and pancreas emergedon the same day of hatching, and thymus was not found until the third day afterhatching. Ontogeny of these immune related organs of the carp in thisresearch is earlier than that reported by Botham.

鲤(Cyprinus carpio)Rh糖蛋白家族基因的克隆与组织mRNA表达

为了研究鱼类氨代谢机制,克隆了鲤(Cyprinus carpio)Rh糖蛋白家族的Rhag、Rhbg、Rhcg1基因的cDNA全序列,与人类Rh基因的氨基酸序列比对结果显示,鲤Rh糖蛋白保守性较高。系统分析表明,鲤3个Rh基因与斑马鱼(Danio rerio)Rh基因的亲缘关系较近。Rhag、Rhbg、Rhcg1基因在鲤鳃组织中表达较高,而在其它组织表达的相对量极低。比较3个基因在鳃组织的表达,Rhbg的表达量极显著高于其它2个基因。这一结果预示Rhag、Rhbg、Rhcg1与鲤的氨代谢密切相关,尤其是Rhbg基因,可能是鲤氨代谢的重要因子。

鲤鱼(cyprinuscarpio)体细胞核移植的初步研究

以黑龙江野鲤的吻端和尾鳍组织为材料进行细胞体外培养，所得原代细胞进行传代，并以传至4～10代的尾鳍继代培养细胞作为供体，以同种鲤及鲫成熟具核未受精卵作为受体，采用显微注射方法进行移核，最终获得了发育至原肠胚期的胚胎．

鲤鱼(Crprinus carpio)体细胞系的建立及其生物学特性分析(简报)

动物细胞的培养技术是1907年哈里逊[1]在淋巴块中对蛙的神经板培养成功开始的,其后近一个世纪以来,陆续成功地培养了哺乳动物、昆虫等各种动物细胞,并广泛用于生物科学的各个分支.鱼类的细胞培养的系统研究和建系实践大约起始于60年代,被公认的真骨鱼类的第一个永久性的细胞系--虹鳟性腺细胞系(RTG-2)是由Wolf[2]建立的.

Cloning and expression analysis in mature individuals of two chicken type-Ⅱ GnRH (cGnRH-Ⅱ) genes in common carp (Cyprinus carpio)

Gonadotropin-releasing hormone (GnRH) is a conservative neurodecapeptide fam-ily, which plays a crucial role in regulating the gonad development and in controlling the final sexual maturation in vertebrate. Two differing cGnRH-II cDNAs of common carp, namely cGnRH-II cDNA1 and cDNA2, were firstly cloned from the brain by rapid amplification of cDNA end (RACE) and reverse transcription- polymerase chain reaction (RT-PCR). The length of cGnRH-II cDNA1 and cDNA2 was 622 and 578 base pairs (bp), respectively. The cGnRH-II pre-cursors encoded by two cDNAs consisted of 86 amino acids, including a signal peptide, cGnRH-II decapeptide and a GnRH-associated peptide (GAP) linked by a Gly-Lys-Arg proteolytic site. The results of intron trapping and Southern blot showed that two differing cGnRH-II genes in common carp genome were further identified, and that two genes might exist as a single copy. The multi-gene coding of common carp cGnRH-II gene offered novel evidence for gene duplica-tion hypothesis. Using semi-quantitative RT-PCR, expression and relative expression levels of cGnRH-II genes were detected in five dissected brain regions, pituitary and gonad of common carp. With the exception of no mRNA2 in ovary, two cGnRH-II genes could be expressed in all the detected tissues. However, expression levels showed an apparent difference in different brain regions, pituitary and gonad. According to the expression characterization of cGnRH-II genes in brain areas, it was presumed that cGnRH-II might mainly work as the neurotransmitter and neuromodulator and also operate in the regulation for the GnRH releasing. Then, the ex-pression of cGnRH-II genes in pituitary and gonad suggested that cGnRH-II might act as the autocrine or paracrine regulator.

Fish Production, Water Quality and Bacteriological Parameters of Koi Carp Ponds Under Live-food and Manure Based Management Regimes

To test the effectiveness of introducing live zooplankton against direct manuring in ornamental fish ponds upon their survival and production, larvae of koi carp, Cyprinus carpio L., were cultured for 11 weeks in earthen ponds maintained according to four management regimes： （1） live zooplankton fed to carp larvae （LF）; （2） direct fertilization with poultry manure （PM）; （3） direct fertilization with cowdung （CD）; and （4） a control treatment （C）. There were three replicates for each treatment. The growth of heterotrophic bacteria and pathogenic microorganisms like Aeromonas sp. and Pseudomonas sp. were also examined in response to pond management. Values of dissolved oxygen were significantly higher （P〈0.05） in the water of LF ponds, compared to other treatments, while the PM and CD treatments recorded were significantly higher （P〈0.05） values of PO4 - P, NH4 - N, NO3 - N, NO2 - N, specific conductivity, alkalinity, and BOD, compared to the LF and C treatments. The percentages of organic carbon and total nitrogen in the bottom sediments were higher in the PM and CD treatments compared to LF （P〈0.05）. Average counts of heterotrophic bacteria in the water of PM and CD ponds were significantly higher than other treatments （P〈0.05）. The development of Aeromonas sp. and Pseudomonas sp. were significantly higher （P〈0.05） in the PM and CD treatments. Weight gain of koi carp stocked in LF was significantly higher （P〈0.05） than that of fish in the other treatments. There was a significant difference in the survival rate of koi carp among the treatments ranging from 67.21% in C to 90.11% in LF. The results suggest that raising koi carp larvae in ponds and feeding them exogenously with zooplankton would support high rates of survival and production through maintenance of better water quality and greater abundance of zooplankton in the system. Significantly lower abundance of Aeromonas sp. and Pseudomonas sp. in the LF treatment considerably lowered any possibility of occurrence of bacterial disease.

苯并芘对鲤鱼胆囊的毒性效应及响应机制

为探讨苯并芘对鲤鱼胆囊的毒理机制,以鲤鱼(Cyprinus carpio)为试验材料,采用15 d慢性毒性试验(苯并芘质量浓度分别为0、0.025和0.25 mg/L),通过检测鲤鱼胆囊中苯并芘质量分数、抗氧化参数、转录应答及免疫基因表达。结果显示:胆囊组织中的苯并芘质量分数积累随着苯并芘胁迫质量浓度显著升高,侧面反映了胆囊在解毒和排毒过程中扮演着重要角色;B[a]P暴露后胆囊抗氧化酶活性(超氧化物歧化酶、过氧化氢酶及谷胱甘肽过氧化物酶)和丙二醛浓度均升高,表明机体可通过激活抗氧化酶系统以应对氧化应激;低质量浓度B[a]P暴露会引起鲤胆囊组织的免疫应答,激活Notch受体信号通路,进而引起细胞凋亡并消除自身组织中过多或异常的细胞;而高质量浓度B[a]P暴露会抑制RIG-I和Notch受体信号通路,引起胆囊免疫稳态失衡,细胞凋亡受到抑制,从而延长异常细胞的存活时间,并进一步激活免疫细胞,导致自身组织的损伤。本研究初步揭示了鲤胆囊细胞应对苯并芘暴露的可能自我保护机制,实现对水环境中多环芳烃污染的早期预警及生态风险评估提供理论基础。

鲤饲料转化率性状的QTL定位及遗传效应分析

数量性状(QTL)定位是实现分子标记辅助育种、基因选择和定位、培育新品种及加快性状遗传研究进展的重要手段。饲料转化率是鲤鱼的重要经济性状和遗传改良的主要目标,而通过QTL定位获得与饲料转化率性状紧密连锁的分子标记以及相关基因是遗传育种的重要工具。研究利用SNP、SSR、EST-SSR等分子标记构建鲤鱼(Cyprinus carpio L.)遗传连锁图谱并对重要经济性状进行QTL定位。选用174个SSR标记、41个EST-SSR标记、345个SNP标记对德国镜鲤F2代群体68个个体进行基因型检测,用JoinMap4.0软件包构建鲤鱼遗传连锁图谱。再用MapQTL5.0的区间作图法(Interval mapping,IM)和多QTL区间定位法(MQMMapping,MQM)对饲料转化率性状进行QTL区间检测,通过置换实验(1000次重复)确定连锁群显著性水平阈值。结果显示,在对饲料转化率性状的多QTL区间定位中,共检测到15个QTLs区间,分布在9个连锁群上,解释表型变异范围为17.70%—52.20%,解释表型变异最大的QTLs区间在第48连锁群上,为52.20%。HLJE314-SNP0919(LG25)区间标记覆盖的图距最小,为0.164 cM;最大的是HLJ1439-HLJ1438(LG39)区间,覆盖图距为24.922 cM。其中区间HLJ1439-HLJ1438、HLJ922-SNP0711解释表型变异均超过50.00%,可能是影响饲料转化率性状的主效QTLs区间。与饲料转化率相关的15个QTLs的加性效应方向并不一致,有3个区间具有负向加性效应,平均为0.027;12个正向加性效应,平均值为0.06。研究检测出的与鲤鱼饲料转化率性状相关的QTL位点可为鲤鱼分子标记辅助育种和更进一步的QTL精细定位打下基础。

鲤鱼乳酸脱氢酶活性的QTL检测

利用SSR分子标记结合"拟测交"策略,以荷包红鲤抗寒品系和柏氏鲤远缘杂交所产生F1代为亲本及其F2代为作图群体,应用Windows Map Manager2.0软件的标记回归法进行乳酸脱氢酶(Lactate dehydrogenase,LDH)活性数量性状基因座单标记定位分析。在乳酸脱氢酶性状的标记回归研究中,共发现12个标记与LDH性状关联,对性状的贡献率为4.00%～10.00%,其中HLJE222达到极显著水平(P<0.01)。为了进一步验证,利用已有的生物信息学工具,将与性状连锁的EST序列与公共数据库中的核酸序列进行同源搜索分析,发现标记HLJE222的EST序列与斑马鱼DAZ associated protein1的mRNA序列相匹配(相似性为94%),与公共数据库中的已知蛋白序列进行相似性比较,同样发现HLJE222的EST与斑马鱼DAZ associated protein1相匹配(相似性为97%)。结果表明HLJE222位点与影响乳酸脱氢酶活性相关的基因连锁。

镜鲤体长、体高、体厚性状QTL定位分析

以镜鲤全同胞家系为材料,用246个SSR和306个SNP标记构建了鲤鱼的连锁图谱,利用GridQTL软件对体长（SL）、体高（H）、体厚（BT）和体长/体高（SLH）进行了QTL定位分析。结果显示：共检测到14个相关的QTL,分布在7个连锁群上。其中,7个与体长相关的QTL——LG6、LG17、LG21、LG23和LG35连锁群上的QTL为显著水平（P〈0.05）,LG1和LG28上达到极显著水平（P〈0.01）,可解释表型变异为6.6%~12.6%;3个与体高相关的QTL均为极显著水平（P〈0.01）位于LG17、LG23和LG28上,可解释表型变异分别为11.6%、12.7%和15.6%;2个与体厚相关的QTL均为显著水平（P〈0.05）位于LG23和LG28上,可解释表型变异分别为8.6%和7.2%;2个与体长/体高相关的QTL均为显著水平（P〈0.05）位于LG21和LG35上,可解释表型变异均为8.2%。

鲤头长、体厚、体高性状的QTL定位及遗传效应分析

用174个SSR、41个EST、345个SNP标记对以镜鲤良种后代为祖父母本所培育的杂交F2群体的68个个体进行基因型检测,运用JoinMap4.0软件包构建遗传连锁图。利用MapQTL5.0区间作图法(interval mapping,IM)和多QTL区间定位法(MQM mapping,MQM)进行QTL检测,通过置换实验(1000次重复)确定连锁群显著性水平阈值。在对体高、头长、体厚的区间定位中,共检测到6个与体高性状相关的QTLs区间,分布在LG1(SNP1339-SNP1490)、LG10(HLJE469-SNP1491)、LG12(SNP0922-HLJ1316)、LG13(SNP0937-HLJ328)、LG25(SNP1041-HLJ594)、LG35(SNP1425-SNP0389)等6个连锁群上,解释表型变异范围为20.0%～43.3%。其中,SNP1339-SNP1490区间LOD值最大为3.64,解释表型变异35.4%。6个与头长相关的QTLs,分布在LG1(SNP1339-SNP1490)、LG12(HLJ071-HLJ336)、LG13(SNP0937-HLJ328)、LG24(SNP1359-SNP0586)、LG24(SNP1016-SNP0326)、LG25(HLJ382-HLJ348)等5个连锁群上,其中LG24(SNP1359-SNP0586)解释表型变异达到50.2%。检测到10个与体厚相关的QTLs,分布在LG1、LG8、LG9、LG10、LG12、LG34、LG35、LG38、LG41等9个连锁群上,解释表型变异范围是16.1%～68.8%,其中LG38(HLJ1331-HLJ487)和LG41(HLJ688-HLJE6)解释表型变异分别达到60.8%和68.8%,是体厚性状的主效QTLs区间。

大豆抗原蛋白Glycinin对鲤稚鱼和幼鱼肠道组织的影响

【目的】研究大豆抗原蛋白大豆球蛋白(Glycinin)对鲤稚鱼、幼鱼肠道组织的影响。【方法】分别以初始体质量为(10.12±0.08)g/尾的鲤稚鱼、(116.89±0.13)g/尾的鲤幼鱼为试验对象,在控温单循环养殖系统中进行饲养试验。以鱼粉为动物蛋白源,混合油脂(m(玉米油)∶m(鱼油)=1∶1)为脂肪源,糊精、面粉作为饲料糖源,分别配制成5种等氮(鲤稚鱼和幼鱼饲料粗蛋白含量分别约为400和360g/kg)等能(总能分别约为16.9和15.2MJ/kg)的半精制饲料,其中大豆抗原蛋白Glycinin的添加量分别为0(对照),30,60,90,120g/kg。每组饲料设3个重复,进行为期8周的饲养试验。饲养试验结束后,采用组织学方法,探讨大豆抗原蛋白Glycinin对鲤稚鱼、幼鱼肠道组织的影响。【结果】在本试验条件下,大豆抗原蛋白Glyicinin添加量为30,60,90,120g/kg组的鲤稚鱼中肠和后肠皱襞高度显著低于对照组(P<0.05);而前肠皱襞高度、肠质量、肠长、肠体指数和肠长指数在各组之间差异不显著(P>0.05)。随着大豆抗原蛋白Glycinin添加量的增加,鲤幼鱼前肠、中肠和后肠皱襞高度呈下降趋势。其中,大豆抗原蛋白Glyicinin的添加量为60,90,120g/kg组鲤幼鱼后肠皱襞高度、肠质量显著低于对照组(P<0.05);而Glyicinin的添加量为120g/kg组鲤幼鱼肠长和肠长指数显著低于对照组(P<0.05);前肠和中肠皱襞高度在各组之间差异不显著(P>0.05)。从肠道形态变化来看,当Glyicinin添加量为60g/kg时,鲤稚鱼肠绒毛开始出现局部断裂或破损;当Glyicinin添加量为90和120g/kg时肠道组织形态进一步被破坏,中肠和后肠受到Glycinin的影响较严重。当Glyicinin添加量为60g/kg时,鲤幼鱼肌层开始出现变薄的现象;当Glyicinin添加量为90和120g/kg时,肠道形态受到的影响较显著,绒毛出现断裂或者缺失。【结论】当鲤稚鱼饲料中大豆抗原蛋白Glyicinin的添加量为30g/kg时,就会引起中肠和后肠皱襞高度下降;而当Glyicinin的添加量为60g/kg时会引起鲤幼鱼后肠皱襞高度下降,同时鲤稚鱼和鲤幼鱼肠道形态开始出现不同程度的破坏。

大豆抗原蛋白Glycinin对鲤稚鱼、幼鱼蛋白酶和淀粉酶活力的影响

【目的】研究大豆抗原蛋白大豆球蛋白(Glycinin)对鲤稚鱼、幼鱼蛋白酶和淀粉酶活力的影响。【方法】以鱼粉为动物蛋白源,混合油脂(m(玉米油)∶m(鱼油)=1∶1)为脂肪源,糊精、面粉为糖源,分别配制大豆抗原蛋白Glycinin添加量为0(CK),30,60,90,120g/kg的5种等氮(稚鱼、幼鱼饲料粗蛋白分别为400和360g/kg)等能(稚鱼、幼鱼饲料总能分别是16.9和15.2MJ/kg)的试验饲料。分别以初始体质量为(10.12±0.08)g/尾的鲤稚鱼和(116.89±0.13)g/尾的鲤幼鱼为试验对象,在控温单循环养殖系统中,进行为期8周的饲养试验,每组饲料设3个重复,探讨大豆抗原蛋白Glycinin对鲤稚鱼、幼鱼蛋白酶和淀粉酶活力的影响。【结果】在鲤稚鱼和幼鱼的配合饲料中,添加不同比例大豆抗原蛋白Glycinin,导致其肠道和肝胰脏蛋白酶活力不同程度下降。其中,鲤稚鱼大豆抗原蛋白Glycinin添加量为30,60,90和120g/kg组的前肠和后肠蛋白酶活力显著低于对照组(P<0.05);而30和60g/kg组中肠和肝胰脏蛋白酶活力与对照组差异不显著(P>0.05),90和120g/kg组中肠和肝胰脏蛋白酶活力显著低于对照组(P<0.05)。在鲤幼鱼配合饲料中,当大豆抗原蛋白Glycinin的添加量为30和60g/kg时,前肠和后肠蛋白酶活力与对照组差异不显著(P>0.05),90和120g/kg组前肠和后肠蛋白酶活力显著低于对照组(P<0.05);而30g/kg组中肠蛋白酶活力与对照组差异不显著(P>0.05),60,90和120g/kg组显著低于对照组(P<0.05);肝胰脏蛋白酶活力各组之间差异不显著(P>0.05)。在本试验条件下,大豆抗原蛋白Glycinin对鲤稚鱼和幼鱼肠道及肝胰脏淀粉酶活力影响不显著(P>0.05)。【结论】在本试验条件下,大豆抗原蛋白Glycinin添加量为30g/kg时,鲤稚鱼前肠和后肠蛋白酶活力显著下降,添加量为60g/kg时,鲤幼鱼中肠蛋白酶活力显著下降,但大豆抗原蛋白Glycinin对鲤稚鱼和幼鱼淀粉酶活力影响不显著。

大豆抗原蛋白Glycinin对鲤稚鱼和幼鱼血液主要生化指标的影响

以初始体质量鲤稚鱼(10.12±0.08)g和鲤幼鱼(116.89±0.13)g为研究对象,利用分离纯化的大豆抗原蛋白Glycinin不同比例(0,3.0%,6.0%,9.0%,12.0%)添加在配合饲料中,以鱼粉为动物蛋白源,糊精、鱼油、玉米油等为能源、纤维素为填充物配制成5种等氮(鲤稚鱼40%,鲤幼鱼36%)、等能(鲤稚鱼16.9 MJ/kg,鲤幼鱼15.2 MJ/kg)的半精制配合饲料,进行为期8周的饲养试验。饲养试验结束后,采用BS400全自动生化分析仪对血液主要生化指标进行测定。结果表明:大豆抗原蛋白Glycinin对鲤稚鱼血液中尿素氮、胆固醇、甘油三酯、血糖、总蛋白、白蛋白、球蛋白、谷草转氨酶、谷丙转氨酶的含量影响不显著(P>0.05)。大豆抗原蛋白Glycinin对鲤幼鱼血液中血糖、总蛋白、白蛋白、球蛋白、谷草转氨酶、谷丙转氨酶的影响不显著(P>0.05),但血液中的尿素氮、胆固醇、甘油三酯的含量随着大豆抗原蛋白Glycinin添加量的增加呈下降趋势,添加量为12.0%组的尿素氮、胆固醇、甘油三酯的含量显著低于对照组(P<0.05)。

镜鲤体长性状的QTL定位分析

以镜鲤良种后代为祖父母本所培育的杂交F2群体的68个个体为材料,利用553个分子标记（217个SSR和336个SNP标记）对其进行基因型检测,运用JoinMap4.0软件包对遗传连锁图谱进行构建。利用MapQTL5.0区间作图法（Interval mapping）进行QTL检测,通过置换实验（1 000次重复）确定连锁群显著性水平阈值。在对体长的区间定位中共检测到12个与体长性状相关的QTLs区间,分布在BL-1-1（SNP0137-SNP1481）、BL-4-1（SNP0092-HLJ797）、BL-5-1（SNP1268-HLJ423）、BL-7-1（HLJ870-SNP0702）、BL-12-1（SNP0922-HLJ639）、BL-16-1（HLJE351-SNP0674）、BL-25-1（SNP0394-SNP0862）、BL-35-1（HLJ668-SNP0832）、BL-43-1（SNP0389-SNP1425）、BL-47-1（HLJ057-HLJ1113）、BL-47-2（HLJ1439-HLJ1418）等11个连锁群上,解释表型变异范围是13.8%~64.9%,其中贡献率大于20%的主效QTLs有8个,是体长性状的主效QTLs区间。

镜鲤体重的QTL定位

本研究利用217个微卫星标记和336个SNPs标记对德国镜鲤F2代68个个体基因组DNA进行基因型检测。其中507个标记共组成62个连锁群,覆盖基因组总长度为2805.85cM,标记间平均距离为6.31cM;利用软件MapQTL4.0采用区间作图法对体重性状进行QTL定位分析。研究结果共检测到14个与体重性状有关的QTLs,分布于9个连锁群。其中BW-5-1有最大的LOD值,为4.46;BW-1-1的LOD值最小,为2.25。单个QTL平均解释表型变异介于14.10%～45.50%之间,其中贡献率大于20%的主效QTLs有9个。通过BLASTX与斑马鱼蛋白质序列数据库进行序列比对,找到了与斑马鱼酰基辅酶A脱氢酶蛋白、胰淀粉酶α2蛋白、Apoeb protein和甘油醛-3-磷酸脱氢酶蛋白同源的分子标记。本研究结果对分子标记辅助育种具有重要应用价值。