一种新的家蚕体形突变体——短体蚕（Sq）的遗传分析与基因定位

作为重要经济昆虫和鳞翅目昆虫模式的家蚕Bombyx mori,其突变体是生理学、遗传学、功能基因组学等研究的宝贵资源。作者在家蚕资源保存和遗传分析中发现一种新的体形突变体——短体蚕（Squab,Sq）,其特征是：杂合体（Sq /+）成活,蚕体长只有正常型的约4/5,腹中部略肥大,胸部稍狭小;纯合体（Sq / Sq）胚胎期致死。遗传分析结果表明该突变为显性遗传。通过与各染色体标记基因进行连锁分析,发现突变基因Sq在家蚕第14染色体上;通过与同一染色体上的标记基因青熟油蚕基因（oa）、不洁蚕基因（Di）进行三点测验,将Sq定位在家蚕连锁图谱第14连锁群的34.6 cM位点,表示为Sq（14-34.6）。本研究结果为深入研究和利用该突变体奠定了重要基础。     

偏执型精神分裂症与4个涉及多巴胺代谢的基因之间的关联分析

精神分裂症是由多基因相互作用导致的复杂疾病。对其易感基因,儿茶酚氧位甲基转移酶基因（COMT）的众多报道充满了矛盾。在对偏执型精神分裂症研究中,我们用多基因座关联分析法研究了4个涉及神经递质多巴胺代谢的基因之间的相互作用。分析结果支持如下假说：COMT-136-BclI对Val^108/158Met有调控作用。当前者的基因型是CC时,后者的易感等位基因型是Met（A）;而当前者的基因型是GG时,后者的易感等位基因型是Val（G）。这一新的假说可以解释此前单基因座分析对Val^108/158Met(COMT)的截然相反的报道,同时也显示了多基因座分析对复杂疾病研究的必要性。      

四种启动子调控RFP报告基因在家蚕细胞(Bm-e-HNU5)内的瞬时表达

以红色荧光蛋白基因（RFP）为报告基因,构建含4种不同启动子的重组表达质粒,用脂质体介导法转染家蚕Bombyx mori细胞（Bm-e-HNU5）,观察家蚕细胞质肌动蛋白4基因启动子（A4）、α微管蛋白基因启动子（α-tub）、蚕丝心蛋白重链基因启动子（Fib）和家蚕核型多角体病毒早期即刻蛋白基因启动子（IE）4种启动子调控RFP报告基因在家蚕细胞内的瞬时表达情况。构建的重组表达质粒pDsRed-α-tub、pDsRed-A4、pDsRed-IE和pDsRed-Fib经双酶切和PCR鉴定正确无误。转染和转录实验结果表明,除了pDsRed-A4外,其他3种重组质粒在Bm-e-HNU5细胞中都得到高转染率,α-tub、IE和Fib可依次增强RFP报告基因在家蚕细胞内的瞬时表达活性。     

家蚕灰色卵的基因所属连锁群的研究（初报）

关于家蚕灰色卵的遗传研究已有许多报 道。到目前为止,已知的有：灰色卵(Gr, 2- 6.9),欧16灰色卵(Gr 16, 2-6.9),淡灰色卵 (GrL,2-6.9), X线诱发灰色卵（Grx-1, 2-6.9 ), 第二X线诱发灰色卵（Grx-a, 2-6.9),斑灰色 卵(mgr, 6-?）及腹白卵(Se, 15-?）等。 日本九州大学农学部家蚕遗传研究所保存 的coil系统的蚕卵卵形正常,卵色灰色,卵 壳呈中度不透明乳白色,是新的自然突变。作 者在此学习期间,就这灰色卵的基因未知所属 连锁群进行了研究,现将结果报告如下     

家蚕细胞周期蛋白基因BmCcnl1的克隆及表达分析

家蚕Bombyx mori由受精卵到完成胚胎发育孵化的过程中, 细胞进行大量的分裂和分化, 然而滞育性卵的胚胎细胞分化至G2期便停滞在此阶段。为了探索这一发育阶段细胞内的分子调控, 本研究以人Homo sapiens的细胞周期蛋白基因cyclin L1为模板, 成功克隆了家蚕同源基因BmCcnl1（GenBank登录号: FJ889988）。BmCcnl1基因开放阅读框（open reading frame, ORF）全长1 254 bp, 编码417个氨基酸。利用Protean软件分析得出BmCcnl1蛋白预测分子量为49 kDa, 等电点为9.84。利用DNA重组技术构建了BmCcnl1基因的重组表达载体pET-21d-BmCcnl1, 对其进行原核表达, 其表达的蛋白以包涵体形式存在。利用RT-PCR技术分析了BmCcnl1基因在胚胎发育过程中的转录水平, BmCcnl1基因在非滞育性卵的胚胎发育阶段基本保持相对稳定的转录表达, 而滞育性卵从蛾体产下经过72 h后已经检测不到BmCcnl1基因的转录。结果提示, BmCcnl1基因与胚胎期滞育及非滞育性卵的发育调控相关。对该基因的克隆和表达分析为今后研究家蚕胚胎发育及细胞周期调控奠定了基础。     

家蚕白卵突变新系BT924的遗传学研究

新的家蚕白色卵突变系BT924是由蓖麻蚕DNA导入家蚕品种苏学5诱导获得。性状特征：滞育卵当年白色,越年后呈浅黄褐色;蛾区内及区间卵色略有变异,幼虫皮肤低度透明,成虫复眼黑色。采用家蚕卵色正常型（黑卵）和突变型红色卵（re）、桃红眼白卵（pe）、第2白卵（w－2）、第3白卵（w－3）及BH863油蚕白卵（w－3bh）与之杂交,进行遗传分析,结果表明,BT924白卵及其油蚕性状由隐性单基因控制,普通遗传,基因座与w－3相同,即：10－19.6。命名为：white egg BT924,基因符号：w－3bt。w－3bt对re表现上位作用。同时发现家蚕基因库保存的桃红眼白卵（pe）标记基因系pe000同时持有红色卵（re）基因,其卵色基因型为re pe/re pe。 Abstract:A new line in white egg mutants of silkworm (Bombyx mori)―BT924 was derived from incorporation of eri?silkworm (Philosamia cynthia ricini Donovan) DAN into the silkworm race “Su Xue 5”.It has the following characteristic traits:The diapause eggs are white in color in the hiberating year and become fawn after hiberation; Slight intra-and inter-batch variation in gee color may exist; Larval skin is slightly translucent; And the compound eyes of the imagos are black.In the present research,the new white egg mutant line was crossed with a normal silkworm race(black egg) and with the mutant lines re,pe,w－2,w－3 and w－3bh for genetical analysis.White egg of BT924 together with its translucency was shown to be controlled by a single recessive gene and share the same locus with w－3(10－19.6). It has been named“white egg BT924”with the gene symbol w－3bt. w－3bt is epistatic to re.In addition,the marker gene line pe000 of pe maintained in the laboratory was shown to carry the re gene as well,its genotype being re pe/re pe.     

即时浸酸显著降低滞育家蚕卵的还原型与氧化型谷胱甘肽比值

即时浸酸在阻止家蚕Bombyx mori卵滞育发动的同时, 显著提高了家蚕卵H₂O₂含量。还原型谷胱甘肽（reduced glutathione, GSH）与氧化型谷胱甘肽（oxidized glutathione, GSSG）的比值是一种氧化胁迫状态的动态指标。为了调查即时浸酸是否造成滞育家蚕卵氧化胁迫, 本研究利用分光光度法分别测定了滞育家蚕卵和5 min即时浸酸滞育家蚕卵中GSH和GSSG含量以及谷胱甘肽转移酶（glutathione-S-transferase, GST）活性。结果表明: 处理后24 h, 即时浸酸处理家蚕卵的总谷胱甘肽（GSH+2GSSG）含量、 GSH含量、 GSSG含量、 GSH/GSSG比值和GST活性分别相当于同期滞育家蚕卵的204%, 78%, 550%, 14%和97%。据此推测, 即时浸酸在阻止滞育发动的同时, 可能通过促进GSH氧化为GSSG, 而显著降低了GSH/GSSG比值, 使家蚕卵处于过氧化状态。     

家蚕血液胰凝乳蛋白酶抑制剂的多态性分布

家蚕Bombyx mori的胰凝乳蛋白酶抑制剂（chymotrypsin inhibitor,CI）在家蚕发育过程中发挥着重要作用,具有丰富的多态性。为了进一步研究家蚕胰凝乳蛋白酶抑制剂在群体水平上的多态性分布,通过非变性聚丙烯酰胺凝胶电泳,调查了425个家蚕品系的血液胰凝乳蛋白酶抑制剂的分布情况。结果表明,基因Ict-A、Ict-D和Ict-E在所有家蚕品系中存在,暗示它们是家蚕正常生长发育必需的基因; 相反,至少在9个家蚕品系中发现基因Ict-B和Ict-H都没有表达,而这些品系没有明显的生理缺陷。在中国品系和日本品系家蚕之间,胰凝乳蛋白酶抑制剂分布规律基本一致。对52个纯品系家蚕的胰凝乳蛋白酶抑制剂分布进行的聚类分析结果表明,胰凝乳蛋白酶抑制剂分布与其系统、眠性和化性都没有明显的相关性。所以家蚕胰凝乳蛋白酶抑制剂广泛存在于不同家蚕品系中,同时多态性的分布特征也表明其生理功能在进化过程中发生了明显的分化。     

西方蜜蜂六个亚种苹果酸脱氢酶Ⅱ基因的遗传差异

研究了西方蜜蜂Apis mellifera 6亚种-浙农大1号意蜂（ZND A. m. ligustica）、东北黑蜂（A. m. ssp.）、卡尼鄂拉蜂（A. m. carnica）、喀尔巴阡蜂（A. m. carpatica）、高加索蜂（A. m. caucasica）和乌克兰蜂（A. m. acervorum）苹果酸脱氢酶Ⅱ的基因型频率、基因频率和杂合纯合度。浙农大1号意蜂、喀尔巴阡蜂和高加索蜂的纯合度较高,但浙农大1号意蜂等位基因c频率最高,喀尔巴阡蜂等位基因b频率最高, 高加索蜂等位基因a频率最高;东北黑蜂、卡尼鄂拉蜂和乌克兰蜂是高度杂合的亚种,但东北黑蜂等位基因a、b、c的频率差异较小,卡尼鄂拉蜂和乌克兰蜂主要存在a、c两个等位基因,b出现频率很小;6亚种的基因型频率、基因频率和杂合纯合度都有极显著差异。这些差异将从遗传和生化角度为西方蜜蜂6个亚种的鉴别提供依据。     

5种中国苏云金芽孢杆菌的伴孢 晶体蛋白基因分析

利用聚合酶联反应(PCR)和聚丙烯酰胺凝胶电泳(SDS-PAGE)技术分析了5种中国苏云金杆菌制剂菌株的伴孢晶体蛋白及其基因组成。结果发现,5种菌株均含有cry1Aa和/或c和/或d和/或b基因,只有Bt+Virus菌株含有cry1Ab基因,cry1A基因编码的伴孢晶体蛋白分子量约为130 kD;仅有JS-Bt C菌株含有cry1B基因,其编码的伴孢晶体蛋白分子量约为138 kD;除HB Bt C菌株外,其余4个菌株均含有cry2Aa和/或b基因,这类基因编码分子量为70 kD的伴孢晶体蛋白;所有5个菌株都含有cry1I基因,其编码的伴孢晶体蛋白分子量应为81.2 kD,但实验中未曾检测到cry1I基因的表达;所有的菌株都不含有cry1C和cry1D基因。     

Molecular basis of the silkworm mutant rel causing red egg color and embryonic death

The coloration and hatchability of insect eggs can affect individual and population survival. However, few genetic loci have been documented to affect both traits, and the genes involved in regulating these two traits are unclear. The silkworm recessive mutant re^l shows both red egg color and embryo mortality. We studied the molecular basis of the re^l phenotype formation. Through genetic analysis, gene screening and sequencing, we found that two closely linked genes, BGIBMGA003497 (Bm-re) and BGIBMGA003697 (BmSema1a), control egg color and embryo mortality, respectively. Six base pairs of the Bm-re gene are deleted in its open reading frame, and BmSema1a is expressed at abnormally low levels in mutant re^l. BmSema1a gene function verification was performed using RNA interference and clustered randomly interspersed palindromic repeats (CRISPR)/CRISPR-associate protein 9. Deficiency of the BmSema1a gene can cause the death of silkworm embryos. This study revealed the molecular basis of silkworm re^l mutant formation and indicated that the Sema1a gene is essential for insect embryo development.     

Chromatic Regulation of Cytochrome Composition and Electron Transfer from Cytochrome b6-f Complex to Photosystem I in Anacystis nidulans (Tx 20)

Cytochrome composition of the cyanobacterial photosyntheticsystem was studied with Anacystis nidulans (Tx 20) in relationto the chromatic regulation of photosystem composition. Comparisonof cytochrome compositions in cells with a high PS I/II ratio(3.0, grown under weak orange light) and with a low ratio (1.6,grown under weak red light) indicated that cytochrome compositionwas also changed in the chromatic regulation of photosystemcomposition. Two types of cytochrome change were observed: 1)contents of cytochromes C₅₅₃ and c₅₄₈ were changed in parallelwith the changes in PS I content, and 2) cytochrome b₅₅₃ andcytochrome b₆-f complex were held at a constant molar ratioto PS II. The molar ratio, PS II : cytochrome b₅₅₉ : cytochromeb₆-f complex : cytochrome c₅₅₃ : PS I : cytochrome C₅₄₈, inthe red-grown cells was 1 : 2.5 : 1.3 : 0.17 : 1.6 : 0.67, andthe ratio in the orange-grown cells, 1:2.4:0.9:0.32:3.0:1.2.In both types of cells, almost all cytochrome f in the cytochromeb₆-f complex was rapidly oxidized after multiple flash activation,indicating that all cytochrome b₆-f complexes in cells of bothtypes are functionally connected to PS I, even when the molarratio to PS I is largely changed. The content of cytochromeC₅₅₃ was at most 0.14 of PS I, suggesting that the cytochrometurns over several times per one turnover of PS I. ¹Present address: Department of Biology, Faculty of Science,Tokyo Metropolitan University, Fukazawa 2-1-1, Setagaya, Tokyo158, Japan. (Received January 20, 1986; Accepted March 17, 1986)     

Pigmentation and Acriflavine Resistance in Serratia marcescens

Stable, orange, acriflavine-resistant variants were selected by treatment of a wild-type, red, acriflavine-sensitive strain of Serratia marcescens with acriflavine. Visible, ultraviolet, infrared, and nuclear magnetic resonance spectra of purified pigment from the red strain were identical to those of the pigment from the orange strain, and the orange mutant was not due to a mutation affecting the structure of the pigment, prodigiosin. The color of the red strain was not affected by variations in pH between 5.0 and 8.0, whereas the color of the orange mutant changed from pink to orange over the same pH range. This variation was mimicked by the pH-induced variation in color of prodigiosin purified from either the red, wild-type or the orange, mutant strains. Density-gradient centrifugation of cell fragments after ultrasonic disintegration resulted in characteristic pigmented bands. Biochemical characterization of these pigmented bands showed that they contained pigment and a protein component, but no lipids, polysaccharides, sugars, glucosamine, or phosphates were detected. Further fractionation of these pigmented bands by zone electrophoresis on a sucrose density gradient indicated that some pigment in S. marcescens was specifically attached to protein components.     

Induced mutation in β-CAROTENE HYDROXYLASE results in accumulation of β-carotene and conversion of red to orange color in pepper fruit

Pepper fruit is typically red, but green, orange and yellow cultivars are gaining consumer acceptance. This color variation is mainly due to variations in carotenoid composition. Orange color in pepper can result from a number of carotenoid profiles, but its genetic basis is only partly known. We identified an EMS-induced orange-fruited mutant using the wild-type blocky red-fruited cultivar ‘Maor’ as progenitor. This mutant accumulates mainly β-carotene in its fruit, instead of the complex pattern of red and yellow carotenoids in ‘Maor’. We identified an A⁷⁰⁹ to G transition in the cDNA of β-CAROTENE HYDROXYLASE2 in the orange pepper and complete co-segregation of this single-nucleotide polymorphism with the mutated phenotype. We therefore hypothesized that β-CAROTENE HYDROXYLASE2 controls the orange mutation in pepper. Interestingly, the expression of β-CAROTENE HYDROXYLASE2 and additional carotenogenesis genes was elevated in the orange fruit compared with the red fruit, indicating possible feedback regulation of genes in the pathway. Because carotenoids serve as precursors for volatile compounds, we compared the volatile profiles of the two parents. The orange pepper contained more volatile compounds than ‘Maor’, with predominant elevation of norisoprenoids derived from β-carotene degradation, while sesquiterpenes predominated in the red fruit. Because of the importance of β-carotene as a provitamin A precursor in the human diet, the orange-fruited mutant might serve as a natural source for pepper fruit biofortification. Moreover, the change in volatile profile may result in a fruit flavor that differs from other pepper cultivars.     

Studies on cytochromes in photosynthetic electron transport system I. photoreduction and photo-oxidation of cytochrome b559 by photosystem II in spinach chloroplasts

Light-induced redox-reactions of cytochrome b₅₅₉ in spinachchloroplasts were investigated. Illumination of chloroplastsinduced photoreduction of cytochrorne b₅₅₉ Red light (650 nm)was more effective than far-red light (725 nm), indicating thatthe photoreduction is a photosystem II-mediated reaction. Onaddition of DCMU, the photoreduction was eliminated and a photooxidationof cytochrome b₅₅₉ was observed. The rate of this photooxidationwas faster with photosystem II light than with photo-systemI light. On addition of Mn⁺⁺ the photooxidation was partly suppressed;far-red light became as effective as red light in inducing photooxidationof cytochrome b₅₉₉, in the presence of DCMU and Mn⁺⁺. Ascorbate completely suppressed photooxidation of cytochromeb⁵⁵⁹ In the presence of ascorbate, however, photooxidation wasobserved in the presence of inhibitors or after inhibitory treatmentsof chloroplasts which affected the oxidizing side of systemII. These inhibitors and inhibitory treatments, but not DCMU,decreased the redoxpotential of cytochrome b₅₅₉. Reactivationof Hill reaction in Tris-washed chloroplasts by indophenol-ascorbatetreatment was not accompanied by an abolishment of photooxidationof cytochrome b₅₅₉. A possible mechanism is proposed to account for these reactionsof cytochrome b₅₅₉ in the photosynthetic electron transportin chloroplasts. (Received April 4, 1972; )     

A comparison of nitrate transport in four different rice (Oryza sativa L.) cultivars

As rice can use both nitrate (NO₃^-) and ammonium (NH₄⁺), we have tested the hypothesis that the shift in the pattern of cultivars grown in Jiangsu Province reflects the ability of the plants to exploit NO₃^- as a nitrogen (N) source. Four rice cultivars were grown in solution culture for comparison of their growth on NO₃^- and NH₄⁺ nitrogen sources. All four types of rice, Xian You 63 (XY63), Yang Dao 6 (YD), Nong Keng 57 (NK) and Si You 917 (SY917), grew well and produced similar amounts of shoot biomass with 1 mmol/L NH₄⁺ as the only N source. However, the roots of NK were significantly smaller in comparison with the other cultivars. When supplied with 1 mmol/L NO₃^-, YD produced the greatest biomass; while NK achieved the lowest growth among the four cultivars. Electrophysiological measurements on root rhizodermal cells showed that the NO₃^--elicited changes in membrane potential (ΔE_m) of these four rice cultivars were significantly different when exposed to low external NO₃^- (<1 mmol/L); while they were very similar at high external NO₃^- (10 mmol/L). The root cell membrane potentials of YD and XY63 were more responsive to low external NO₃^- than those of NK and SY917. The ΔE_m values for YD and XY63 rhizodermal cells were almost the same at both 0.1 mmol/L and 1 mmol/L NO₃^-; while for the NK and SY917 the values became larger as the external NO₃^- increased. For YD cultivar, ΔE_m was measured over a range of NO₃^- concentrations and a Michaelis-Menten fit to the data gave a K_m value of 0.17 mmol/L. Net NO₃^- uptake depletion kinetics were also compared and for some cultivars (YD and XY63) a single-phase uptake system with first order kinetics best fitted the data; while other cultivars (ND and SY917) showed a better fit to two uptake systems. These uptake systems had two affinity ranges: one had a similar K_m in all the cultivars (0.2 mmol/L); the other much higher affinity system (0.03 mmol/L) was only present in NK and SY917. The expression pattern of twelve different NO₃^- transporter genes was tested using specific primers, but only OsNRT1.1 and OsNRT2.1 expression could be detected showing significant differences between the four rice cultivars. The results from both the physiological and molecular experiments do provide some support for the hypothesis that the more popular rice cultivars grown in Jiangsu Province may be better at using NO₃^- as an N source.     

Phenotypic analysis of conditionally immortalized cells isolated from the BPK model of ARPKD

To study the pathophysiology ofautosomal recessive polycystic kidney disease (ARPKD), we soughtto develop conditionally immortalized control and cystic murinecollecting tubule (CT) cell lines. CT cells were isolated fromintercross breedings between BPK mice(bpk^+/), a murine model of ARPKD,and the Immorto mice(H-2K^b-ts-A58^+/+).Second-generation outbred offspring (BPK × Immorto) homozygous for the BPK mutation (bpk^/;Im^+/±; cysticBPK/H-2K^b-ts-A58), were phenotypicallyindistinguishable from inbred cystic BPK animals(bpk^/). CysticBPK/H-2K^b-ts-A58 mice developed biliary ductalectasia and massively enlarged kidneys, leading to renal failure anddeath by postnatal day 24. Principal cells (PC) wereisolated from outbred cystic and noncystic BPK/H-2K^b-ts-A58 littermates at specificdevelopmental stages. Epithelial monolayers were under nonpermissiveconditions for markers of epithelial cell polarity and PC function.Cystic and noncystic cells displayed several properties characteristicof PCs in vivo, including amiloride-sensitive sodium transport andaquaporin 2 expression. Cystic cells exhibited apical epidermal growthfactor receptor (EGFR) mislocalization but normal expression of ZO-1 and E-cadherin. Hence, these cell lines retain the requisitecharacteristics of PCs, and cysticBPK/H-2K^b-ts-A58 PCs retained the abnormal EGFRmembrane expression characteristic of ARPKD. These cell lines representimportant new reagents for studying the pathogenesis of ARPKD.

     

Effects of Salinity on Some Citrus Scion-Rootstock Combinations

Chloride and sodium concentrations, water relations and gasexchange parameters were measured on leaves of Clementine (CitrusClementine Hort. ex. Tan) and Navel orange [C. sinensis (L.)Osb] scions grafted on Cleopatra mandarin (C. reticulata Blanco)and Troyer citrange (C. sinensis x Poncirus trifoliata) rootstocksgrown at increasing levels of NaCl in the external medium. Otherparameters affected by salinity such as growth and defoliationwere also recorded. Scions on Cleopatra mandarin accumulated less Cl^- in their leavesthan did scions on Troyer citrange. Also, leaf Cl^- levels inClementine scions were lower than in Navel orange when bothwere grafted on the same rootstock. However, sodium concentrationwas lower in scions on Troyer citrange than in Cleopatra mandarin. Leaf water potential, stomatal conductance, photosynthesis andgrowth were reduced more in grafted plants of salt-treated Navelorange than those of salt-treated Clementine. However, choiceof rootstock had little effect on salt-induced changes in theseparameters. For each scion, reduction in leaf stomatal conductancewas closely correlated with decrease in leaf water potential.Also, a significant correlation between photosynthesis and stomatalconductance was found. The results indicate that reductions in gas exchange parametersand growth at increasing salinity levels depended more on thescion type than on Cl^- or Na⁺ concentration in leaves. Otherwise,leaf injury and defoliation were closely correlated with leafCl^- concentration.Copyright 1995, 1999 Academic Press Citrus, photosynthesis, salinity, water relations     

褐飞虱对噻嗪酮抗性的遗传分析

害虫的抗性遗传特性是影响其抗性发展的一个重要因子,也是制订抗性治理对策的重要依据。我们采用稻茎浸渍法测定了褐飞虱Nilaparvatalugens (Stal)抗性和敏感亲本、正反交（F₁、F₁₂、F'₂）及回交（BC）后代3龄若虫对噻嗪酮的剂量反应数据,研究了褐飞虱对噻嗪酮的抗性遗传特性。结果表明: 正反交后代的显性度分别为-0.3153（F₁）和-0.376 3（F'₁）,表明抗性遗传为常染色体的不完全隐性;将自交及回交后代的剂量反应数据进行单个主基因假设的卡方(χ²)检验,其卡方值分别为42.11（F₂）、5.44 （F'₂）及93.57（BC）,均大于χ^２0.05= 15.51(df=8),表明其抗性是多基因控制的。还讨论了褐飞虱对噻嗪酮的抗性治理策略。