多花水苋对苄嘧磺隆的抗性水平及靶标抗性机制

为明确水稻田杂草多花水苋Ammannia multiflora对乙酰乳酸合成酶 (ALS) 抑制剂类除草剂苄嘧磺隆的抗性水平和抗性分子机制,采用整株水平测定法,测定了采自江苏省扬州市田间的多花水苋疑似抗性种群 (YZ-R) 对苄嘧磺隆的抗性指数,并分析了YZ-R种群和相对敏感种群 (YZ-S)多花水苋ALS酶对苄嘧磺隆的敏感性差异,同时比较了YZ-R和YZ-S种群ALS基因的核苷酸序列差异。结果表明:YZ-R种群多花水苋对苄嘧磺隆已表现出高水平抗性,其抗性指数 (RI) 为40.6;苄嘧磺隆对YZ-R种群ALS酶活性的抑制中浓度 (I₅₀) 为0.087 μmol/L,对YZ-S种群的I₅₀值为0.0028 μmol/L,其抗性指数为31.1。通过PCR扩增获得了多花水苋ALS基因的部分序列,该序列包含了已报道的8个氨基酸突变位点。ALS基因序列比对分析发现,YZ-R种群多花水苋植株ALS基因第197 位氨基酸由脯氨酸 (CCT) 突变为丝氨酸 (TCT)。研究表明,ALS基因发生脯氨酸 (Pro)-197-丝氨酸 (Ser) 的突变,导致多花水苋ALS酶对苄嘧磺隆的敏感性下降,是多花水苋YZ-R种群对苄嘧磺隆产生高水平抗性的主要原因。     

稻田雨久花对苄嘧磺隆的抗药性

性指数达63.4;对德惠抗、感雨久花ALS活力的IC50分别为10 756.2和396.8nmol/L,抗性指数为27.1.表明两地稻田雨久花均对苄嘧磺隆产生了抗药性,而其体内ALS敏感性降低是产生抗药性的原因之一.     

抗苄嘧磺隆野慈姑乙酰乳酸合成酶的突变研究

近年来,野慈姑Sagittaria trifolia L.在中国东北稻区发生和危害日趋严重,部分稻区使用苄嘧磺隆已无法有效防除该杂草。为了明确野慈姑抗药性发生的根本原因,本试验从分子水平上对野慈姑抗苄嘧磺隆的机理进行了研究。通过对抗药性(H4)和敏感性(S)野慈姑种群靶标酶乙酰乳酸合成酶(ALS)基因片段进行扩增和克隆,比较其DNA序列的差异,确定导致抗药性产生的ALS氨基酸突变位点。结果表明,与敏感性野慈姑ALS基因相比,H4种群第197位脯氨酸(Pro)突变为苏氨酸(Thr),该位点的突变可能是H4野慈姑种群对苄嘧磺隆产生抗药性的主要原因。ALS第197位Pro突变为Thr致使对苄嘧磺隆产生抗药性是第一次在野慈姑种群中报道。     

抗精噁唑禾草灵和甲基二磺隆看麦娘ACCase和ALS基因突变

为明确看麦娘Alopecurus aequalis抗性种群YL的靶标抗性机制,采用基因克隆法对看麦娘抗性和敏感种群间乙酰辅酶A羧化酶(ACCase)和乙酰乳酸合成酶(ALS)基因序列进行扩增、克隆和测序,比对二者ACCase和ALS基因序列的差异,探寻其产生抗药性突变的基因位点,同时测定该突变型抗性种群YL对不同ACCase和ALS抑制剂类除草剂的交互抗性。结果显示,与看麦娘敏感种群TL相比,抗性种群YL的ACCase基因CT区域第2 041位氨基酸由异亮氨酸(ATT)突变为天冬酰胺酸(AAT),ALS基因Domain A区域第197位氨基酸由脯氨酸(CCC)突变为精氨酸(CGC)。看麦娘抗性种群YL对ACCase抑制剂炔草酯产生了高水平抗性,抗性倍数为43.96,对高效氟吡甲禾灵和精喹禾灵产生了中等水平抗性,抗性倍数分别为18.33和15.87,对唑啉草酯、烯草酮和烯禾啶较敏感;对ALS抑制剂氟唑磺隆产生了低水平抗性,抗性倍数为8.39,对啶磺草胺和咪唑乙烟酸较敏感。表明ACCase基因第2 041位和ALS基因第197位氨基酸突变是导致看麦娘抗性种群YL对精噁唑禾草灵和甲基二磺隆同时产生抗性的重要原因之一。     

河南省部分地区麦田荠菜对苯磺隆的抗性水平及抗性靶标分子机制

为明确河南省部分地区麦田荠菜Capsella bursa-pastoris对苯磺隆的抗性水平及抗性靶标分子机制,采用整株生物法测定了12个荠菜种群的抗性水平,并对乙酰乳酸合成酶(acetolactate synthase,ALS)离体活性和ALS基因突变进行了测定分析。结果表明,商丘市民权县花园村(MQ)、周口市西华县小于楼村(XH)、平顶山市叶县穆寨村(YX)、许昌市长葛市董庄村(CG)采集的荠菜种群对苯磺隆产生了较高的抗性,GR_(50)分别为129.14、110.67、62.91和85.29 g/hm~2,抗性倍数分别为215.23、184.45、104.85和142.15倍;ALS离体活性测定所得I_(50)分别为5.85、4.87、1.38和3.83μmol/L,抗性倍数分别为83.57、69.57、19.71和54.71倍;其余8个种群的GR_(50)在0.60~2.86 g/hm~2之间,抗性倍数在1.00~4.77之间;I_(50)在0.07~0.37μmol/L之间,抗性倍数在1.00~5.29之间。荠菜种群MQ、XH的ALS基因Domain A区域第197位脯氨酸(CCT)均突变为丝氨酸(TCT),荠菜种群CG的第197位脯氨酸(CCT)突变为亮氨酸(CTT),表明靶标ALS基因突变是荠菜对苯磺隆产生抗性的重要原因之一,但荠菜种群YX的ALS基因保守区内暂未发现突变位点,其抗药性可能由其它原因造成。     

耳叶水苋对乙酰乳酸合成酶抑制剂的抗性及其分子机制初探

近年来长江下游地区稻田耳叶水苋Ammannia arenaria H.B.K.危害十分严重。采用盆栽法首次测定了耳叶水苋对苄嘧磺隆等药剂的抗性水平,同时分析了其抗性和敏感种群间乙酰乳酸合成酶(ALS)基因的DNA序列及其RNA表达差异。结果表明:采自浙江嘉兴(JX110)、江苏苏州(JS039)、浙江宁波(NB0143-05)和安徽广德(AH014)的耳叶水苋生物型对苄嘧磺隆的抗性指数(RI)分别为67.90、17.59、44.63和8.37,对苄嘧磺隆表现出中高水平抗性的生物型对五氟磺草胺、双草醚及咪唑乙烟酸也产生了低水平的抗性。获得了耳叶水苋ALS基因全长核苷酸序列2235 bp,编码667个氨基酸,仅发现NB0143-05等3种抗性生物型ALS酶的氨基酸序列非保守区第93位的亮氨酸被脯氨酸取代。然而,NB0143-05的ALS酶对ALS抑制剂的敏感性大幅度降低(RI 37.04),且在苄嘧磺隆处理后4 d的ALS基因表达量是敏感生物型(HZ001)的1.86倍。这表明,ALS酶对药剂的敏感性降低以及被苄嘧磺隆诱导后ALS基因表达量显著增加,很可能是耳叶水苋生物型NB0143-05对ALS抑制剂产生抗性的原因。     

玉米田反枝苋对烟嘧磺隆的抗性水平及靶标抗性分子机理

为明确玉米田主要杂草反枝苋对烟嘧磺隆的抗性水平及靶标抗性分子机理,采用整株水平测定法检测了黑龙江省玉米田反枝苋对烟嘧磺隆的抗性水平,通过靶标酶离体活性测定,分析了抗性和敏感种群反枝苋乙酰乳酸合成酶 (ALS) 对烟嘧磺隆的敏感性,并通过靶标ALS基因克隆测序进行了序列比对分析。结果显示:黑龙江省反枝苋疑似抗性种群 (HLJ-R) 对烟嘧磺隆已产生较高水平抗性,其抗性倍数达13.7;酶活性测定结果表明:烟嘧磺隆对HLJ-R种群ALS活性的抑制中浓度 (IC₅₀) 值是对敏感种群 (TA-S) IC₅₀值的43.9倍;与TA-S种群相比,HLJ-R种群ALS基因205位丙氨酸突变为缬氨酸,574位色氨酸突变为亮氨酸。研究表明,黑龙江省玉米田反枝苋对烟嘧磺隆已产生较高水平抗性,且靶标ALS基因的突变可能是其抗性产生的主要原因之一。     

麦田抗性生物型荠菜对苯磺隆的抗性机制研究

为明确抗性生物型荠菜对苯磺隆的抗性机制,分别测定了苯磺隆对抗性和敏感生物型荠菜体内乙酰乳酸合成酶(ALS)、谷胱甘肽-S-转移酶(GSTs)、超氧化物歧化酶(SOD)、过氧化物酶(POD)和过氧化氢酶(CAT)的影响。结果表明:离体条件下,抗性生物型荠菜体内ALS对苯磺隆的敏感性明显降低,苯磺隆对荠菜抗性和敏感生物型ALS的抑制中浓度(I50)分别为0.722 8和0.052 1 μmol/L,抗性与敏感生物型I50的比值为13.87;活体条件下,施用苯磺隆后,抗性和敏感生物型荠菜ALS活性均受到一定程度的抑制,但抗性生物型ALS活性受到抑制后能逐渐恢复,而敏感生物型则不能恢复;经苯磺隆处理后,抗性生物型GSTs相对活力明显高于敏感生物型,而抗性和敏感生物型体内POD、SOD和CAT相对活力无明显差异。研究表明,抗性生物型荠菜体内ALS对苯磺隆敏感性降低是其抗药性产生的原因之一,而GSTs对苯磺隆代谢能力的差异也可能与荠菜对苯磺隆的抗性有关。     

黑龙江省稻田野慈姑对丙嗪嘧磺隆抗性相关研究

通过整株盆栽法研究黑龙江省佳木斯市汤原县(种群R1)、856农场(种群R2)、密山市(种群R3)3个水稻田野慈姑种群对丙嗪嘧磺隆的抗性水平,采用分子生物学技术分析3个野慈姑种群在靶标酶基因上的差异,确定3个野慈姑种群对丙嗪嘧磺隆和苄嘧磺隆是否存在交互抗性。结果显示,黑龙江R1、R2、R3种群抗性指数(RI)分别为11.92、22.68、35.99。与敏感的七台河种群S相比,R1、R2、R3的ALS基因均在Pro_(197)位发生不同突变。R1种群为Thr_(197)取代了Pro_(197);R2、R3种群为Ser_(197)取代了Pro_(197),ALS基因的突变是其产生抗性的主要原因。3个野慈姑种群对丙嗪嘧磺隆和苄嘧磺隆存在交互抗性。     

宁夏地区稗草种群对五氟磺草胺的抗性机制研究

为了明确宁夏稻区稗草对五氟磺草胺抗性水平及抗性机制。采用整株生物测定法测定了宁夏地区6个稗的原变种Echinochloa crus-galli var.crus-galli种群对五氟磺草胺的抗性水平,并测定了每个种群的乙酰乳酸合酶基因(ALS)序列和ALS酶离体活性,以及P450抑制剂马拉硫磷对稗草种群抗性水平的影响。结果显示,与敏感种群相比,5个疑似抗性种群对五氟磺草胺表现出不同程度的抗性(10.18倍～32.71倍),其中抗性种群N14,N22,N27和N51的ALS 574位色氨酸突变为亮氨酸,N53的197位脯氨酸突变为亮氨酸,敏感种群N43没有发现突变位点,五氟磺草胺对抗性种群ALS酶的IC₅₀均明显高于敏感种群,马拉硫磷对五氟磺草胺有增效作用,可提高稗草种群对五氟磺草胺的敏感性。综上所述,稗草种群对五氟磺草胺产生抗性是由于靶标基因ALS突变,同时稗草种群对五氟磺草胺的抗性也可能与细胞色素P450介导的代谢增强有关。     

Mechanism of resistance to bensulfuron-methyl in Alisma plantago-aquatica biotypes from Portuguese rice paddy fields

Two Alisma plantago‐aquatica biotypes resistant to bensulfuron‐methyl were detected in rice paddy fields in Portugal’s Mondego (biotype T) and Tagus and Sorraia (biotype Q) River valleys. The fields had been treated with bensulfuron‐methyl‐based herbicide mixtures for 4–6 years. In order to characterize the resistant (R) biotypes, dose–response experiments, absorption and translocation assays, metabolism studies and acetolactate synthase (ALS) activity assays were performed. There were marked differences between R and susceptible (S) biotypes, with a resistance index (ED₅₀R/S) of 500 and 6.25 for biotypes Q and T respectively. Cross‐resistance to azimsulfuron, cinosulfuron and ethoxysulfuron, but not to metsulfuron‐methyl, imazethapyr, bentazone, propanil and MCPA was demonstrated. No differences in the absorption and translocation of ¹⁴C‐bensulfuron‐methyl were found between the biotypes studied. Maximum absorption attained 1.12, 2.02 and 2.56 nmol g⁻¹ dry weight after 96 h incubation with herbicide, for S, Q and T biotypes respectively. Most of the radioactivity taken up by the roots was translocated to shoots. Bensulfuron‐methyl metabolism in shoots was similar in all biotypes. The R biotypes displayed a higher level of ALS activity than the S biotype, both in the presence and absence of herbicide and the resistance indices (IC₅₀R/S) were 20 197 and 10 for biotypes Q and T respectively. These data confirm for the first time that resistance to bensulfuron‐methyl in A. plantago‐aquatica is target‐site‐based. In practice, to control target site R biotypes, it would be preferable to use mixtures of ALS inhibitors with herbicides with other modes of action.     

Occurrence of sulfonylurea resistance in Sagittaria trifolia,a basal monocot species,based on target‐site and non‐target‐site resistance

Sagittaria trifolia L. is one of the most serious weeds in paddy fields in Japan. Since the late 1990s, severe infestations of S. trifolia have occurred following applications of sulfonylurea herbicides in Akita prefecture. In this study, two accessions of S. trifolia, R1 and R2, were collected from paddy fields with severe infestations and their resistance profiles were determined in comparison to a susceptible accession, S1. R1 and R2 were highly resistant to bensulfuron‐methyl. R1 was also highly resistant to pyrazosulfuron‐ethyl, but R2 was susceptible. Relative to S1, R1 had an amino acid substitution at the Pro₁₉₇ residue of acetolactate synthase (ALS), a well‐known mutation that confers sulfonylurea resistance, suggesting that R1 has a target‐site‐based resistance (TSR) mechanism. The sequence of the ALS gene in R2 was identical to that in S1. A Southern blot analysis indicated that there was only one copy of the ALS gene in S1 and R2. These results suggest that R2 has a non‐target‐site‐based resistance (NTSR) mechanism. R2 was moderately resistant to imazosulfuron but susceptible to thifensulfuron‐methyl. R2 and S1 were susceptible to pretilachlor, benfuresate, MCPA‐ethyl and bentazon. The results reveal the occurrence of two sulfonylurea‐resistant biotypes of S. trifolia that show different mechanisms of cross‐resistance to sulfonylureas related to TSR in R1 and NTSR in R2.     

Mutations of the ALS gene endowing resistance to ALS-inhibiting herbicides in Lolium rigidum populations

BACKGROUND: In the important grass weed Lolium rigidum (Gaud.), resistance to ALS‐inhibiting herbicides has evolved widely in Australia. The authors have previously characterised the biochemical basis of ALS herbicide resistance in a number of L. rigidum biotypes and established that resistance can be due to a resistant ALS and/or enhanced herbicide metabolism. The purpose of this study was to identify specific resistance‐endowing ALS gene mutation(s) in four resistant populations and to develop PCR‐based molecular markers. RESULTS: Six resistance‐conferring ALS mutations were identified: Pro‐197‐Ala, Pro‐197‐Arg, Pro‐197‐Gln, Pro‐197‐Leu, Pro‐197‐Ser and Trp‐574‐Leu. All six mutations were found in one population (WLR1). Each Pro‐197 mutation conferred resistance to the sulfonylurea (SU) herbicide sulfometuron, whereas the Trp‐574‐Leu mutation conferred resistance to both sulfometuron and the imidazolinone (IMS) herbicide imazapyr. A derived cleaved amplified polymorphic sequences (dCAPS) marker was developed for detecting resistance mutations at Pro‐197. Furthermore, cleaved amplified polymorphic sequences (CAPS) markers were developed for detecting each of the six mutant resistant alleles. Using these markers, the authors revealed diverse ALS‐resistant alleles and genotypes in these populations and related them directly to phenotypic resistance to ALS‐inhibiting herbicides. CONCLUSION: This study established the existence of a diversity of ALS gene mutations endowing resistance in L. rigidum populations: 1–6 different mutations were found within single populations. At field herbicide rates, resistance profiles were determined more by the specific mutation than by whether plants were homo‐ or heterozygous for the mutation. Copyright © 2008 Society of Chemical Industry     

Transformation a mutant Monochoria vaginalis acetolactate synthase (ALS) gene renders Arabidopsis thaliana resistant to ALS inhibitors

Acetolactate synthase (ALS) genes from Monochoria vaginalis resistant (R) and susceptible (S) biotypes against ALS inhibitors found in Korea revealed a single amino acid substitution of Proline (CCT), at 169th position based on the M. vaginalis ALS sequence numbering, to serine (TCT) in conserved domain A of the gene (equal to the proline 197 in Arabidopsis thaliana ALS gene sequence). A. thaliana plants transformed with the single mutated (Pro₁₆₉ to Ser) M. vaginalis ALS gene (including transit signal peptide) showed cross-resistance patterns to ALS-inhibiting herbicides, like as sulfonylurea-herbicide bensulfuron methyl (R/S factor of 9.5), imidazolinone-herbicide imazapyr (R/S factor of 5.1), and triazolopyrimidine-herbicide flumetsulam (R/S factor of 17.6) when measuring hypocotyls’ length of A. thaliana. The ALS activity from the transgenic A. thaliana plants confirmed the cross-resistance pattern to these herbicides like as R/S factor of 8.3 to bensulfuron methyl, 2.3 to imazapyr, and 13.2 to flumetsulam.     

Resistance levels of sulfonylurea‐resistant Schoenoplectus juncoides (Roxb.) Palla with various Pro197 mutations in acetolactate synthase to imazosulfuron,bensulfuron‐methyl,metsulfuron‐methyl and imazaquin‐ammonium

An investigation, using herbicidal pot tests in a greenhouse condition, was conducted to determine the whole‐plant dose–response relationships to several acetolactate synthase (ALS)‐inhibiting herbicides of sulfonylurea (SU)‐resistant Schoenoplectus juncoides with various Pro₁₉₇ mutations in ALS that was collected from Japanese rice paddy fields. All the tested SU‐resistant accessions with a Pro₁₉₇ mutation were highly resistant to two commonly used SU herbicides (imazosulfuron and bensulfuron‐methyl), but were much less resistant to another SU herbicide, metsulfuron‐methyl, and were substantially not resistant to imazaquin‐ammonium. These cross‐resistance patterns have been known previously in fragments of S. juncoides and other weed species and were comprehensively confirmed in this study with a whole set of Pro₁₉₇ mutations. The analyses of resistance levels, based on ED₉₀ values, newly showed that different accessions with a common amino acid substitution in ALS1 showed similar responses to these herbicides (confirmed with four amino acid substitutions), that the rankings of resistance levels that were conferred by various Pro₁₉₇ mutations in ALS1 differed among the SU herbicides and that the resistance levels of the ALS2‐mutated accessions were higher than, lower than or similar to those of the corresponding ALS1‐mutated accessions, depending on the compared pair, but the deviation patterns were generally similar among the SU herbicides in each compared pair. The final finding might suggest that the abundance of ALS2 is not as stable as that of ALS1. In addition, as a result of these new findings, together with expected further research, a suggested possibility is that substituting amino acids at Pro₁₉₇ generally could be estimated by plotting each accession's ED₉₀ values of imazosulfuron and bensulfuron‐methyl in a two‐dimensional graph.     

Inheritance of sulfonylurea resistance in Monochoria vaginalis

The inheritance of sulfonylurea (SU) resistance in Monochoria vaginalis was investigated based on the bensulfuron‐methyl response phenotypes of F₁ plants between SU‐resistant (R) and ‐susceptible (S) and segregation analysis in F₂ progenies. Differences of SU resistance between SU‐R biotypes and F₁ plants at the recommended field dose were also investigated by comparing shoot dry weight. All F₁ plants survived the treatment with 25 g a.i. ha^?1 bensulfuron‐methyl, one‐third of the recommended field dose, and showed similar responses to SU‐R plants. Conversely, all F₁ plants died or showed extreme necrosis at 225 g a.i. ha^?1, three times the recommended field dose, as SU‐S plants. F₂ plants were classified as either R or S phenotype. Segregation for resistance to bensulfuron‐methyl in F₂ families did not differ from the expected 3:1 (R:S) ratio at 25 g a.i. ha^?1. At 225 g a.i. ha^?1, the F₂ families segregated in a 1:3 (R:S) ratio. These results suggest that SU resistance in M. vaginalis is controlled by a single nuclear allele with resistance being dominant at low dose and susceptibility dominant at high dose. Moreover, F₁ plants died or were extremely injured after application of bensulfuron‐methyl at the recommended field dose, although SU‐R biotypes grew normally.     

0.2%苄嘧磺隆·丙草胺颗粒剂在水稻田中的残留及消解动态

采用高效液相色谱（HPLC）法研究了0.2%苄嘧磺隆·丙草胺颗粒剂在稻田环境中的消解动态和最终残留。稻田水、谷壳、稻秆和水稻植株样品用二氯甲烷提取,土壤样品用V（二氯甲烷）:V（甲醇）=9:1的混合液提取,糙米样品用V（二氯甲烷）:V（甲醇）=7:3的混合液提取后再用二氯甲烷萃取;HPLC法测定。结果表明:当添加水平在0.05~1 mg/kg（或mg/L）时,苄嘧磺隆和丙草胺的平均回收率均在75%~103%之间,相对标准偏差（RSD）为1.6%~13%;苄嘧磺隆和丙草胺的检出限（LOD）均为0.02 mg/L,最小检出量均为4.0×10-10 g,在稻田水中的最低检测浓度（LOQ）均为0.001 mg/L,在稻田土壤中的LOQ均为0.005 mg/kg,在水稻植株、谷壳和糙米中的LOQ均为0.01 mg/kg。在水稻移栽后5~7 d,采用直接撒施法在高剂量（270 kg/hm2,其中苄嘧磺隆有效成分为67.5 g/hm2,丙草胺有效成分为472.5 g/hm2）下施药1次的消解动态试验结果表明:在稻田水、土壤和水稻植株中,苄嘧磺隆的消解半衰期分别为5.06~5.83 d、9.76~11.55 d和4.52~4.82 d,丙草胺的消解半衰期分别为5.94~6.45 d、7.70~9.90 d和4.11~4.89 d。分别按低剂量（180 kg/hm2,其中苄嘧磺隆有效成分为45 g/hm2,丙草胺有效成分为315 g/hm2）和高剂量（270 kg/hm2）施药1次,在正常收获期收获的糙米中均未检出苄嘧磺隆和丙草胺残留。     

Resistance of Rotala indica Koehne var. uliginosa Koehne to sulfonylurea herbicides

The present paper aims to quantify the degree of resistance development in Rotala indica Koehne var. uliginosa Koehne to sulfonylurea (SU) herbicides based on whole plant responses. Seeds of resistant (from Omagari City, Akita Prefecture, Japan) and susceptible (from Tsukuba City, Ibaraki Prefecture, Japan) R. indica plants were seeded in 200 cm² pots. The plants, at the 1.5 leaf stage, were blanket-applied with different rates of three sulfonylurea herbicides: bensulfuron methyl (BSM), pyrazosulfuron ethyl (PSE) and imazosulfuron (ISN). Of the three herbicides, the weed appears to have developed the highest degree of resistance to BSM. The resistant/susceptible (R/S) values based on mortality, root length and dry weight are consistently highest at 197, 157 and 101, respectively. Responses based on shoot length, however, showed a higher R/S value for PSE. Roots of R. indica are more sensitive to higher rates of SU herbicides than the shoots. Indeed, a high degree of resistance to SU herbicides have evolved in R. indica , for which the recommended field rates are not enough for effective control of the weed.