铜绿假单胞菌噬菌体的分离鉴定及耐噬菌体突变频率测定*

用铜绿假单胞菌为宿主菌自污水中分离到3株不同的铜绿假单胞菌噬菌体,命名为PaP1、PaP2及PaP3者均为DNA双链噬菌体,基因组大小分别约为47kb、34kb及24kb。3株噬菌体原液滴度（pfu）分别为10⁹/mL、10¹¹/mL和10¹¹/mL。PaP1为裂菌性噬菌体,PaP2及PaP3为溶原性噬菌体。电镜观察,3株噬菌体头部均为多面体立体对称颗粒,直径分别约为70nm、55nm和65nm。PaP1属肌尾噬菌体科,PaP2和PaP3属     

一株可裂解动物源性多重耐药志贺氏菌的噬菌体分离鉴定及其生物学特性研究

从鸡的肠道内分离鉴定多重耐药志贺氏菌(Shigelle)，纯化获得可侵袭、裂解该志贺氏菌的噬菌体，并研究其生物学特性。以养殖场病鸡肠道中分离的志贺氏病原菌为宿主，筛选鉴定噬菌体，聚乙二醇沉淀浓缩噬菌体，通过透射电镜观察噬菌体形态，双层平板法测定噬菌体宿主谱、最佳感染复数、一步生长曲线、酸碱耐受性和热稳定性，测定噬菌体对多重耐药致病性志贺氏菌的裂解效果。通过上述方法，共筛选到26株志贺氏菌分离株，分别命名为BS1~BS26。以志贺氏菌BS26为宿主菌分离得到一株裂解性噬菌体并命名为噬菌体PSF26，鉴定为有尾噬菌体目，长尾噬菌体科，噬菌体对福氏志贺氏菌（Shigella flexneri）和宋内志贺氏菌(Shigella sonnei)分离株均有裂解作用。噬菌体PSF26的最佳感染复数为0.1，感染周期为90 min，包括75 min的潜伏期和15 min的爆发期，裂解量为(58±17) pfu/cell。噬菌体PSF26在pH 5~8，温度0~40 ℃条件下能保持较高活性，对宿主菌的抑菌圈直径为(11.33±1.53) mm。结果表明，噬菌体PSF26爆发期短，裂解量高，有较好的酸碱、温度耐受性，对多重耐药性福氏和宋内志贺氏菌有良好的作用效果，为利用噬菌体防控饲养动物中食源性致病菌感染和饲用抗生素替代技术研发提供参考。     

五株克雷伯氏菌噬菌体的生物学特性及比较基因组学研究

【目的】耐药性克雷伯氏菌属(Klebsiella)的细菌作为人类感染的重要病原,是临床治疗重要的挑战。本研究对多株克雷伯氏菌裂解性噬菌体的生物学特性和基因组特征进行比较分析,为其应用提供更多科学数据。【方法】使用双层平板法从人类和动物新鲜粪便、污水中分离纯化裂解性克雷伯氏菌噬菌体;通过磷钨酸染色和透射电镜观察其形态;采用双层平板噬菌斑法确定其宿主范围,测定温度和pH稳定性、一步生长曲线和体外抑菌效果等生物学特性;基于全基因组测序对分离株进行比较基因组学分析;通过体内抑菌试验评估噬菌体对多重耐药变栖克雷伯氏菌(Klebsiella variicola) BS375-3感染的大蜡螟(Galleria mellonella)幼虫的保护作用。【结果】5株噬菌体分别属于Schitoviridae (pKP-BM327-1.2)、Autographiviridae (pKP-M186-2.1、pKP-M186-2.2和pKV-BS375-3.1)、Drexlerviridae (pKP-BS317-1.1)家族;噬菌体pKV-BS375-3.1可裂解受试菌中的8株,pKP-BM327-1.2可裂解受试菌中的3株,pKP-M186-2.1、pKP-M186-2.2和pKP-BS317-1.1则分别裂解受试菌中的1株;5株噬菌体感染10-20 min后即进入指数增长期,在-20-37 ℃、pH 6-10环境下均能够保持稳定活性;感染变栖克雷伯氏菌BS375-3后经噬菌体pKV-BS375-3.1处理[感染复数(multiplicity of infection, MOI)=100]的大蜡螟幼虫96 h内存活率达到80% (8/10);5株噬菌体基因组长度在42-77 kb之间,未携带抗生素抗性基因和毒力基因,基于内溶素(endolysin)的溯源分析显示该蛋白在克雷伯氏菌噬菌体中呈现多样性,属内呈保守性。【结论】5株克雷伯氏菌噬菌体均具有较好的体外抑菌活性,生物学特性稳定,endolysin在噬菌体属内呈现保守性。宿主谱宽、潜伏期短的噬菌体pKV-BS375-3.1在治疗Klebsiella pneumoniae和K. variicola临床感染方面具有潜在应用前景。     

布氏菌噬菌体SA对各种布氏菌的裂解活性

布氏菌噬菌体SA是从猪种布氏菌培养物中分离到的。其裂解活性当菌液浓度为10^-4时,对光滑型猪种菌1、3型,牛种菌1、3、6型和沙林鼠种菌可产生混合性裂解,产生噬菌斑直径3—4mm。噬菌体SA原液或稀释浓度为10^-1、10^-2时,对羊种菌1、3型不裂解。对羊种菌2型、粗糙型牛种菌45/20、犬种菌和绵羊附睾菌产生混合性裂解或噬菌斑,噬菌斑为1—2mm或更小。     

噬菌体phiYe-F10的裂解谱的测定以及裂解能力与宿主毒力基因间关系分析

目的为测定小肠结肠炎耶尔森菌噬菌体phiYe-F10的裂解谱,分析噬菌体phiYe-F10裂解能力与宿主毒力基因间的关系。方法采用双层平板法观察噬菌体phiYe-F10对213株小肠结肠炎耶尔森菌,36株假结核耶尔森菌和1株鼠疫耶尔森菌的裂解能力;同时对不同来源不同地区的小肠耶尔森菌进行黏附侵袭位点基因(ail)、肠毒素基因(ystA、ystB)、黏附素基因A(yadA)、毒力因子基因F(virF)、O∶3血清型特异性基因(rfbc)检测和血清型别鉴定。结果表明213株小肠结肠炎耶尔森菌包括O∶3血清型84株(其中rfbc+78株),O∶5血清型10株,O∶8血清型13株,O∶9血清型34株,其它及未分型的共72株。携带毒力质粒的典型致病性小肠耶尔森菌(ail+,ystA+,ystB-,yadA+,virF+)77株,毒力质粒丢失的致病性小肠结肠炎耶尔森菌(ail+、ystA+、ystB-、yadA-、virF-)15株,其它非致病基因型121株。噬菌体phiYe-F10裂解71株O∶3小肠结肠炎耶尔森氏菌,其中致病性小肠结肠炎耶尔森菌52株,非致病性小肠结肠炎耶尔森菌19株。对O∶5,O∶9血清型和其它菌株均不裂解,对O∶3的裂解率高达84.5%(71/84)。噬菌体phiYe-F10对假结核耶尔森菌和鼠疫耶尔森氏菌均不裂解。结论:phiYe-F10噬菌体是一株小肠结肠炎耶尔森菌的裂性噬菌体,在25℃时表现出一个典型的窄裂解谱,高度专一性裂解O∶3血清型小肠结肠炎耶尔森菌。phiYe-F10对典型致病性小肠结肠炎耶尔森菌的裂解能力明显高于非致病性的小肠结肠炎耶尔森菌     

应用肠杆菌科四个属的诊断噬菌体快速诊断沙门氏菌

本文报告应用弗氏柠檬酸细萄噬菌体3组,大肠埃希氏菌噬菌体4组,阴沟肠杆菌噬菌体1组和沙门氏菌O-I噬菌体快速诊断沙门氏菌的结果。沙门氏菌0-I噬菌体可裂解沙门氏菌属地方株1393株中的1351株(97％)。柠檬酸细菌属噬菌体和共可裂解柠橡酸细菌属地方株381株中的362株(95％)。阴沟肠杆菌噬菌体Ent可裂解阴淘肠杆菌地方株l 50株中的133株(84．2％)。埃希氏菌属噬菌体E—1、E一2、E-3和E-4共可裂解埃希氏菌属地方株683株中的567株(83％)。由于E一1和E一2噬菌体的联合使用,可使o I噬菌体对埃希氏菌属地方株的误诊率从6．3％下降到0．6％。E一4噬菌体对沙门氏菌属地方株的误诊率可因与。一I噬菌体的联合使用而从0．36％下降到0．07％。     

副溶血弧菌噬菌体Vpas_PP24的分离鉴定及生物学特性

【背景】副溶血弧菌是南美白对虾养殖中常见的致病菌,传统的抗生素防治办法不仅低效,而且越来越难以满足食品安全和绿色环保及可持续发展的要求。副溶血弧菌的生物防治是南美白对虾养殖业可持续发展的必由之路。噬菌体是天然安全的活体抗菌剂,因其对特定细菌的专一性感染和高效性裂解而备受关注。【目的】分离一株能高效裂解副溶血弧菌的烈性噬菌体,为探索副溶血弧菌的噬菌体防治方法提供基础研究。【方法】以28株病虾来源的副溶血弧菌为宿主菌,用双层琼脂平板法从海鲜市场污水中分离副溶血弧菌噬菌体;点斑法测定噬菌体的裂解谱,并对筛选到的宽裂解谱噬菌体进行透射电镜(transmission electron microscopy,TEM)观察、生物学特性测定和全基因组序列分析。【结果】分离筛选到一株副溶血弧菌烈性噬菌体,命名为Vpas_PP24。透射电镜观察显示该噬菌体头部为二十面体,有一长尾,头部长约92 nm,宽约46 nm,尾部长约147 nm,属于有尾噬菌体目长尾噬菌体科。其基因组全长83 482 bp,预测有118个开放阅读框(open reading frames,ORFs),具有已知功能的有13个,不含非编码RNA、毒力基因及抗生素抗性基因。基因组一致性对比显示噬菌体Vpas_PP24可能为弧菌噬菌体的一个新种。Vpas_PP24对28株副溶血弧菌的裂解率为54%,对其他种属的116株弧菌的总裂解率为16%;最佳感染复数(multiplicity of infection,MOI)为0.000 1,效价可达3.0×10¹⁰ PFU/mL。一步生长曲线显示Vpas_PP24的潜伏期为10 min,暴发期为150 min,暴发量为30 PFU/cell。该噬菌体在温度<50 ℃、pH 4.0-11.0范围内活性稳定,对糜蛋白酶、木瓜蛋白酶和对虾肝胰腺酶提取液的水解作用不敏感,但蛋白酶K可快速使其失活,紫外辐照也能使Vpas_PP24失活。宿主菌对该噬菌体的不敏感突变频率为2×10^-5。【结论】分离筛选到一株裂解谱较宽、基因型较新、生物学性质较稳定的副溶血弧菌噬菌体,该噬菌体具有进一步开发成为新型副溶血弧菌抗菌剂的潜力。     

用荧光标记O-I噬菌体快速检测食品源沙门氏菌

[目的]利用O-I噬菌体几乎可裂解沙门氏菌属细菌的特性建立快速检测食品中沙门氏菌的方法.[方法]用核酸荧光染料SYBR gold染料标记O-I噬菌体侵染100株试验菌及120份食品样品菌,荧光显微镜鉴定沙门氏菌;并测灵敏度.[结果]100株试验菌中40株沙门氏菌可见杆状荧光,而10株变形杆菌、20株志贺氏菌、20株大肠杆菌和10株葡萄球菌均无荧光;沙门氏菌检测灵敏度达10 CFU/100 μL;120份食品样品中沙门氏菌的O-I噬菌体检测与生化鉴定结果的阳性率分别为9.17%和10%,符合率为91.7%.[结论]试验表明用荧光标记的O-I噬菌体可以快速、直观、准确、大量地检测食品中沙门氏菌.     

深圳赤潮中霍乱弧菌噬菌体的分离筛选及生物学特性分析

本文以从鲍鱼肠道中分离出的霍乱弧菌SWBC-a为宿主菌,采用双层平板法从2004年夏季深圳大梅沙海域赤潮海水样品中分离得到10株噬菌体。通过对分离出的噬菌体效价、RTD值的测定、形态特征的观察及对属内外细菌的交叉裂解谱的研究,筛选出3株裂解谱较宽的强效噬菌体。选取其中2株高效裂解噬菌体PsaA和PsaH做生物学特性分析,证明除镁离子有利于噬菌体裂解外,温度、pH值、紫外照射、柠檬酸钠对噬菌体裂解都有不同程度的抑制。本研究结果为进一步利用噬菌体研发用于消除霍乱弧菌的微生态制剂和诊断食源性霍乱弧菌提供了理论基础。     

朱鹮肠道微生物多样性与产酶活性

【背景】朱鹮是我国国家一级保护动物,属于世界上最濒危的鸟类之一。对朱鹮肠道微生物的多样性和产胞外酶活性进行分析,可为朱鹮种群数量恢复提供思路。【目的】了解朱鹮肠道微生物的多样性,测定其产胞外酶活性。【方法】采用纯培养的方法获得朱鹮肠道微生物,通过革兰氏染色和生理生化鉴定,结合16S rRNA基因扩增和序列分析对细菌进行鉴定。使用水解圈法筛选产淀粉酶、蛋白酶、纤维素酶、脂肪酶的菌株。【结果】从人工喂养的朱鹮新鲜粪便中共分离到296株细菌,共计2个门11个属。变形菌门(Proteobacteria) 236株,占分离总数的79.73%,分别为：埃希氏菌属(Escherichia) 137株,占分离总数的46.28%;哈夫尼亚菌属(Hafnia) 39株,占分离总数的13.18%;变形菌属(Proteus) 28株,占分离总数的9.46%;柠檬酸杆菌属(Citrobacter) 23株,占分离总数的7.77%;气单胞菌属(Aeromonas) 6株,占分离总数的2.03%;肠杆菌属(Enterobacter) 1株,占分离总数的0.34%;志贺菌属(Shigella) 1株,占分离总数的0.34%;克雷伯菌属(Klebsiella) 1株,占分离总数的0.34%。厚壁菌门(Firmicutes) 60株,占分离总数的20.27%,分别为：肠球菌属(Enterococcus) 33株,占分离总数的11.15%;库特氏菌属(Kurthia) 14株,占分离总数的4.73%;芽孢杆菌属(Bacillus) 13株,占分离总数的4.39%。优势菌群为变形菌门(Proteobacteria)中的埃希氏菌属(Escherichia),占细菌总数的46.28%。经过生理生化鉴定,每个菌株生理生化鉴定出的种属与各自的16S rRNA基因鉴定出的种属相一致。产酶活力分析结果显示有238株产蛋白酶、25株产脂肪酶、24株产淀粉酶、15株产纤维素酶,分别占分离总数的80.41%、8.45%、8.11%和5.07%。【结论】朱鹮肠道微生物分离出的细菌可分为2门11属,优势菌群为变形菌门(Proteobacteria)中的埃希氏菌属(Escherichia),占细菌总数的46.28%;产酶活性分析显示,80.41%的菌株具有产蛋白酶能力。     

Bacteriophage Typing of Proteus mirabilis, Proteus vulgaris, and Proteus morganii

A bacteriphage typing scheme for differentiating Proteus isolated from clinical specimens was developed. Twenty-one distinct patterns of lysis were seen when 15 bacteriophages isolated on 8 Proteus mirabilis, 1 P. vulgaris, and 1 P. morganii were used to type 162 of 189 (85.7%) P. mirabilis and P. vulgaris isolates. Seven phages isolated on 3 P. morganii were used to type 13 of 19 (68.4%) P. morganii isolates. Overall, 84.1% of the 208 isolates were lysed by at least 1 phage at routine test dilution (RTD) or 1,000 x RTD. Fifty isolates, retyped several weeks after the initial testing, showed no changes in lytic patterns. The phages retained their titers after storage at 4 C for several months. A computer analysis of the data showed that there was no relationship between the source of the isolate and bacteriophage type. This bacteriophage typing system may provide epidemiological information on strains involved in human infections.     

Predominance of phage group II in Staphylococcus strains isolated from humans

2545 strains of Staphylococcus aureus isolated from 24 Polish laboratories in the years 1994-95 were investigated. Phage typing was performed according to the method of Blair and Williams using the present basic set of typing phages and additional phages 88, 89 and 187. The phages were employed in concentrations of RTD and 100 x RTD. The predominance of phage group II, reported elsewhere since 1980-ties, was found in the present study (23.6%). Strains of group III were second in frequency (16.6%), whereas strains of groups I and V, as well as type 95 occurred in small percentage (7.6%, 4% and 3.4% respectively). Strains of groups II and V have been rarely lysed by phages belonging to other groups. The use of additional phages resulted in typability of strains by 7.9%. Percentage of non-typable strains was high and amounted to 22.0%.     

Coagulase-negative Staphylococci isolated from patients. III. Phage typing

Coagulase-negative staphylococci of clinical origin were subjected to phage typing by means of phages from the experimental Dutch (Verhoef) and American (Paris) sets. These sets of phages were used to study 153 and 378 strains, respectively. The Dutch phages could lyse 30.1%, and the American ones 19.6% of the cultures. The strains belonging to the species S. epidermidis were lysed in 34.3% and 32.4% of cases, respectively, which is indicative of the fact that the American phages possess a more pronounced specificity in respect to S. epidermidis. The unsufficient effectiveness of typing phages does not yet allow one to evaluate the outlook for the method of phage typing in the study of coagulase-negative staphylococci.     

Evaluation of the usefulness of three collections of bacteriophages for typing methicillin-resistant Staphylococcus aureus,isolated in Moscow hospitals

The typing of S. aureus methicillin-resistant strains, isolated in different hospitals of Moscow; was carried out with the use of three collections of phages: the International Set of Phages; the set of phages of the International Center of S. aureus phage typing in London (L); and the experimental collection of phages of the Gamaleya Institute of Epidemiology and Microbiology in Moscow (M). In this study made with the use of both the phages of the International Diagnostic Set and phages L in the standard typing dose of 1 TP about 6% of the cultures under study proved to be sensitive. When the typing dose was increased to 100 TP the phages of the international diagnostic set lyzed 75.5% of the cultures. The typed strains were found to belong to phage types 77 (71.7%), 77/84/85 (19.6%) and 94/96 (6.5%). At a concentration of 100 TP phages L lyzed 83.7% of the cultures, but the dominating phage types could not be determined due to a great variety of phage markers. In contrast to the two preceding collections, the third phage collection M was composed in such a way that in the study of the investigated culture the specificity of its restriction modification was primarily evaluated and only then the presence of antiphage immunity was determined. This latter collection was used in the evaluation of 93.1% of the cultures. By the specificity of their restriction specification system the majority of them were classified with two new groups, heretofore not described. Only this collection M made it possible to differentiate epidemic and sporadic strains and to evaluate the epidemic situation in all 6 hospitals.     

Radiation Treatment of Foods: II. Public Health Significance of Irradiation-Recycled Salmonella1

Salmonellae resistant to gamma irradiation were developed by repeated irradiation and subculturing in a nutrient broth-yeast extract medium. Few differences were noted in the biochemical characteristics of parent and resistant cultures; however, microculture studies revealed variations in morphology and in cell division patterns. A considerable decrease in pathogenicity for day-old chicks was apparent with resistant cultures, but their phenol-water extracts were as toxic as parent material for 10-day chick embryos. Five serial chick passages did not reverse the reduced pathogenicity or aberrant morphology of a resistant Salmonella typhimurium culture. Results of phage typing of both parent and serially irradiated S. typhimurium were inconclusive, whereas the O-1 genus-specific phage lysed all parent serotypes tested but only one of the serially irradiated cultures. Agglutination of parent S. typhimurium cells with their homologous rabbit antiserum was unaffected by prior absorption with resistant strains. The results indicate that radiation recycling altered Salmonella into strains of lesser public health significance.     

Bacteriophage Typing as an Epidemiological Tool for Urinary Escherichia coli

Phage typing was used to identify strains of Escherichia coli isolated from urinary and nonurinary sources. When eight phages isolated in Pennsylvania were used to type 717 cultures from Missouri, 50.3% of 624 urinary isolates and 34.4% of 93 nonurinary isolates were typable. Strains from nonurinary sources were not found commonly in urine. When five additional phages isolated in Missouri were added to the original set of eight phages, 80.4% of 331 urinary isolates were typable. When this set of phages was used to type 552 urinary cultures isolated in California, Minnesota, Ohio, Pennsylvania, Virginia, and West Virginia, 82.0% of the cultures were typable. Some common phage types were found in high incidence among cultures from the different regions. No correlation was found between phage type and the pattern of resistance to antibiotics. Phage typing data were presented also on the number of strains in individual urine specimens and the recurrences of strains in patients with chronic bacteriuria. Of 97 fecal isolates, 75.2% of the cultures were typable, and the most common phage type was observed in high incidence among the urinary isolates from this region. When 75 cultures from nine other genera of enteric bacteria were typed, only the shigellae were lysed. In view of the information obtained by phage typing and the ease and speed with which it can be done, it is suggested that phage typing be considered a new tool in epidemiological studies of urinary tract infections by E. coli.     

Bacteriophage Types and O Antigen Groups of Escherichia coli from Urine

Urinary strains of Escherichia coli from seven geographical regions were typed serologically for O-specific antigens and with phages capable of lysing the majority of urinary isolated. The O antigen groups 4, 6, 75, 1, 50, 7, and 25 were the common ones found. Of the 454 cultures tested, 66.1% were phage typable and 65.2% were serotypable with the 48 antisera employed. Also, 71.6% of the cultures for which an O group could be determined were phage typable. Furthermore, of those seven O-antigen groups implicated in urinary tract infection, 80.2% exhibited a phage pattern. Various phage types were found within an O-antigen group, and, although one phage type associated a high percentage of the time with one O-antigen group, no correlation was observed between other O-antigen groups and phage types. Studies with bacteriuric patients by phage typing showed the presence of two strains of E. coli within an O-antigen group. Serogrouping and phage typing of fecal isolates of E. coli revealed the presence of some O-antigen groups and phage types also found as predominant types among urinary isolates. Phage typability correlated highly with hemolysis of human erythrocytes. Elevated temperatures of incubation and a chemical curing agent were used to enhance typability of cultures refractory to the typing phages. Phage typing, due to its rapidity, ease, and ability to distinguish strains of E. coli within an O-antigenic group, is suggested as a possible method by which a better insight into the epidemiology of urinary tract infections may be obtained.     

Incidence and properties of temperate bacteriophages induced from lactic streptococci.

Sixty-three strains of lactic streptococci isolated from commercial lactic streptococcal starter cultures were examined for lysogeny by treatment with ultraviolet light or mitomycin C. After treatment with the inducing agent, all strains, whether or not they lysed, were examined for evidence of phage release by electron microscopy. Thirty-eight strains yielded intact phages or phage particles of varying morphology. All the temperate phages had isometric heads and noncontractile tails; some had collars and structurally distinctive baseplates. Indicator host strains were found for phages induced from seven different strains. Three strains that released phages spontaneously yielded titers of 10(3) to 10(4) plaque-forming units per ml. When strains that spontaneously released phages were grown in mixed culture with indicator strains, increased phage titers of 10(6) to 10(7) plaque-forming units per ml were observed. These findings indicate that lysogenic lactic streptococcal strains may serve as a reservoir for phages that attack sensitive strains in mixed- or multiple-strain lactic starter cultures.     

Incidence and properties of temperate bacteriophages induced from lactic streptococci.

Sixty-three strains of lactic streptococci isolated from commercial lactic streptococcal starter cultures were examined for lysogeny by treatment with ultraviolet light or mitomycin C. After treatment with the inducing agent, all strains, whether or not they lysed, were examined for evidence of phage release by electron microscopy. Thirty-eight strains yielded intact phages or phage particles of varying morphology. All the temperate phages had isometric heads and noncontractile tails; some had collars and structurally distinctive baseplates. Indicator host strains were found for phages induced from seven different strains. Three strains that released phages spontaneously yielded titers of 10(3) to 10(4) plaque-forming units per ml. When strains that spontaneously released phages were grown in mixed culture with indicator strains, increased phage titers of 10(6) to 10(7) plaque-forming units per ml were observed. These findings indicate that lysogenic lactic streptococcal strains may serve as a reservoir for phages that attack sensitive strains in mixed- or multiple-strain lactic starter cultures.     

Phage types of Staphylococcus aureus strains and their antibiotic resistance in carriers of medical students population

The phage types of 78 S. aureus strains isolated from nose swabs obtained from a medical students in 2005 -2006 was determined and antibiotic resistance of the phage types was analysed. 680 students were tested in order to obtain the strains and 11.5% of them were carriers of S. aureus. Phage typing was performed using basic set of23 phages and 3 additional phages: 88, 89 and 187. Drug resistance was determined by the disc-diffusion method. The most frequent in studied population were the group III (21.8%) and strains lysed by phages belonging to varied groups (21.8%). Highly different phage patterns were observed among strains belonging to each of the group. Strains belonging to the group III as the strains lysed by phages from varied groups were most frequently resistant only to penicillin (52,9% respectively). Resistance to penicillin was also most often observed in the strains belonging to another groups and phage types. Usefulness of the additional phages 88,89 and 187 was in the investigations as no more than 51% of strains was lysed by this phages.