JPS6257306B2 - - Google Patents

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Publication number
JPS6257306B2
JPS6257306B2 JP58149378A JP14937883A JPS6257306B2 JP S6257306 B2 JPS6257306 B2 JP S6257306B2 JP 58149378 A JP58149378 A JP 58149378A JP 14937883 A JP14937883 A JP 14937883A JP S6257306 B2 JPS6257306 B2 JP S6257306B2
Authority
JP
Japan
Prior art keywords
seaweed
enzyme solution
hydrolase
protoplasts
polysaccharide
Prior art date
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
Expired
Application number
JP58149378A
Other languages
Japanese (ja)
Other versions
JPS6041485A (en
Inventor
Teruhiko Shibata
Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)
KOASA SHOJI KK
Original Assignee
KOASA SHOJI KK
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by KOASA SHOJI KK filed Critical KOASA SHOJI KK
Priority to JP58149378A priority Critical patent/JPS6041485A/en
Publication of JPS6041485A publication Critical patent/JPS6041485A/en
Publication of JPS6257306B2 publication Critical patent/JPS6257306B2/ja
Granted legal-status Critical Current

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  • Cultivation Of Seaweed (AREA)
  • Micro-Organisms Or Cultivation Processes Thereof (AREA)

Description

【発明の詳现な説明】[Detailed description of the invention]

本発明は、海苔の健党なプロトプラストを調補
する方法、曎に詳しくは、现胞融合に有効に適甚
し埗る海苔のプロトプラストを調補する方法に関
する。 近幎、遺䌝子工孊的手法ずしお異皮生物䜓の现
胞間の融合、いわゆる现胞融合に぀いおの研究が
非垞に盛んずなり、陞䞊怍物においおは既に実甚
化の段階にたで成功したものもみられるに至぀お
いる。 しかしながら、海藻類、特にアマノリ類に関し
おの现胞融合の研究報告は少なく、その成功䟋に
぀いおも未だみられおいない。 因に、コムギ、オオムギ、倧豆などの陞䞊怍物
では垂販の酵玠剀䟋えばセルラヌれ、マセロチ
ヌム等を甚いお容易にそれらのプロトプラスト
を調補し埗るけれども、アマノリ類をプロトプラ
スト化できる酵玠が珟圚のずころ入手し埗ないた
め、アマノリ類の现胞融合の技術が陞䞊怍物に比
べお遅れおいる䞀因ず考えられる。 而しお、アマノリ類をプロトプラスト化するた
めの詊みずしおは今たでのずころ、藀田等による
「酵玠凊理によるノリ、アオノリ類のプロトプラ
ストの分離ずその発生」に぀いおの報告日本氎
産孊䌚、昭和57幎秋季講挔芁旚集、第23頁、
213がみられるのみである。この藀田等による
方法は、海苔葉䜓を物理的手段で现断しお埗られ
る葉片にシナヌドモナスPseudomonasSPの
菌株―株の培逊液から埗た粗酵玠液を玄
時間皋床䜜甚させおプロトプラストを調補する
ものであるが、この方法ではプロトプラストを埗
るための酵玠凊理に長時間を芁し、しかも海苔を
物理的に切断したものに酵玠を䜜甚させるので埗
られるプロトプラストが䞍健党になる可胜性が高
く、したが぀おこのプロトプラストを甚いおの现
胞融合に支障をきたすおそれがある。蓋し、现胞
融合の手法においおはそれに甚いるプロトプラス
トの健党床が非垞に䞻芁な芁因であ぀お、プロト
プラストが䞍健党であるず现胞融合に圓぀おの融
合率が䜎くな぀お以埌の培逊による生育も劣るよ
うになるず考えられるからである。 たた、䞊蚘方法で海苔葉䜓を切断するのは、シ
ナヌドモナスSP菌株が生産する酵玠が海苔の衚
局郚分には䜜甚せずに切断郚分から䜜甚しお海苔
の现胞壁を厩壊しおプロトプラストずなるずの認
識に基づいおいるものず考えられる。 Preston等の報告によるず、海苔は衚局にマン
ナンが顆粒状に存圚しおおり、海苔の现胞壁はミ
クロフむブリル圢態のキシランから構成されおお
り、现胞充間物質ずしおポルフむランが存圚しお
いるずされる。たた、L.A.Hanic等によるず、海
苔の衚局には蛋癜質から成る薄い被芆が存圚しお
いるずされる。すなわち、このような海苔の組識
䞊の芳点から、海苔は切断しなければプロトプラ
スト化できないず考えられおいたものず思われ
る。 本発明者は、现胞融合に適した海苔の健党なプ
ロトプラストを埗るには、海苔を物理的に切断す
るこずなくその衚局から厩壊させるこずが必芁で
あるずの芋地から海苔のプロトプラスト化に぀い
お怜蚎した結果、海苔を少なくずもマンナン加氎
分解酵玠およびキシラン加氎分解酵玠を含有する
酵玠液で凊理するか、曎にはポリフむラン加氎分
解酵玠も含有する酵玠液で凊理するこずにより、
海苔のプロトプラストを健党な状態で調補し埗る
こずの知芋を埗お本発明をなすに至぀た。 すなわち、本発明の目的は、现胞融合に有効に
適甚し埗る海苔の健党なプロトプラストを調補す
る方法を提䟛するこずにある。 以䞋本発明を詳しく説明する。 本発明の構成䞊の䞻芁な特城は、海苔葉䜓を、
シナヌドモナス属に属する難消化性倚糖類の加氎
分解胜を有する埮生物を、海苔もしくは海苔由来
の倚糖類を誘導物質ずしお含む培地䞭で培逊しお
埗られる培逊液から調補される少なくずもマンナ
ン加氎分解酵玠ずキシラン加氎分解酵玠を含有す
る酵玠液で凊理するこずにある。なお、本発明の
其他の構成は以䞋の説明から明らかになるであろ
う。 本発明で海苔のプロトプラスト化に甚いる酵玠
液の調補に利甚される難消化性倚糖類の加氎分解
胜を有する埮生物は、海氎䞭から分離されたもの
であ぀お、䞊蚘倚糖類であるマンナン、キシラン
およびポルフむランの加氎分解胜を有し、䞋蚘の
ずおりの菌孊的性質を有する。 菌孊的性質 圢態 ZoBELL2216E培地に生育した现胞に぀い
お、 (ã‚€) 现胞の圢態は桿菌では倧きさは0.5〜Ό
×1.5〜2.5Ό (ロ) 運動性を有し、鞭毛は単極毛性 (ハ) グラム染色性は陰性 生育状態 ZoBELL2216E斜面培地における生育状態、 (ã‚€) 20℃〜27℃の枩床で良奜に生育する (ロ) 淡黄色の色玠を沈着 (ハ) 毛状filiformの集萜を圢成 生理孊的性質 (ã‚€) カタラヌれテスト 陜性 (ロ) オキシダヌれテスト 陜性 (ハ) グルコヌスよりの酞の生成 陜性 (ニ) ―テストHugh Leifson法による
 (ホ) Vibro―Static Agent129 陰性 (ヘ) 塞倩液化胜  (ト) キシラン分解胜  (チ) マンナン分解胜  (リ) 奜気性 䞊蚘菌孊的性質に鑑み、本発明で利甚する䞊蚘
埮生物はシナヌドモナス属Pseudomonasに
属する菌株であるず同定し埗る。なお、この菌株
シナヌドモナスPseudomonassp.PT―は埮
工研条寄第330号の受蚗番号で工業技術院埮生物
工業技術研究所に寄蚗されおいる。 本発明では䞊蚘埮生物を、海苔もしくは海苔由
来の倚糖類を誘導物質ずしお含む培地䞭で培逊し
おマンナン加氎分解酵玠、キシラン加氎分解酵玠
曎にはポルフむラン加氎分解酵玠を培地䞭に生産
する。 ここで甚いる“海苔由来の倚糖類”ずは海苔を
熱氎抜出しお可溶性成分を陀去しお埗られる、䞻
ずしお倚糖類から成る残枣、又は該残枣を曎に粟
補凊理しお倚糖類含量を高めたものを意味する。 䟋えば、海苔を10倍量の氎に浞挬し、オヌトク
レヌブ䞭で120℃で30分間加熱したのち、濟垃を
甚いお可溶性区分を陀去し、埗られる残枣に぀い
お䞊蚘ず同様の手順で加熱しお可溶性区分を陀去
する操䜜を繰返し行い回皋床、぀いで埗ら
れる残枣を100゚タノヌルに浞挬し、宀枩にお
䞀倜攟眮したのち、可溶性区分を陀去し、也燥し
たものを倚糖類から成る残枣ずしお甚いるか、又
は、䞊蚘加熱ず可溶性区分の陀去を繰返し行぀お
埗られる残枣゚タノヌル浞挬を行぀おいないも
のを1N―NaOH溶液に浞挬し、宀枩にお䞀倜攟
眮したのち、可溶性区分を陀去した残枣をNaOH
の20熱氎溶液で抜出し、埗られる抜出液を遠心
分離し、その䞊柄液にプヌリング溶液を加えお
沈柱を生成させ、この沈柱物を氎掗しおCuむオ
ンを陀去しお埗られる倚糖類マンナンもしく
は䞊蚘プヌリング溶液を加えお沈柱を生成させ
たずきの䞊柄液にHC1を加えおPHをに調敎しお
埗られる沈柱物から成る倚糖類キシランをそ
れぞれ粟補凊理した倚糖類ずしお甚いる。 䞊蚘誘導物質ずしおの海苔もしくは海苔由来の
倚糖類の培地に察する添加量は乃至重量が
適圓である。 本発明で利甚する䞊蚘埮生物の培逊に甚いる培
地は、炭玠源ずしお䞊蚘誘導物質を、窒玠源ずし
おペプトンおよび酵母゚キスを、曎に無機質ずし
おK2HPO4、FeCl3などを海氎又は人工海氎に溶
解し、緩衝液䟋えばトリス緩衝液でPHを7.5前
埌に調敎したものが奜たしい。培地組成を䟋瀺す
るず䞋蚘のずおりである。 培地組成 海苔又は海苔由来の倚糖類 1.0重量 ペプトン 1.0 酵母゚キス 0.1 K2HPO4 0.01 FeCl3 0.6mg トリス緩衝液 0.1重量 䞊蚘割合で海氎に溶解しおPHを7.5に調敎す
る。 本発明で利甚する䞊蚘埮生物の䞊蚘培地におけ
る培逊条件は、25℃の枩床で日間通気、撹拌通
気䞋通気量1000〜2000mlmin、撹拌数100〜
300r.p.m.に行う。 䞊述のようにしお培逊しお埗られた培逊液から
酵玠液を調補するには、該培逊液を℃の枩床で
30分間遠心分離10000r.p.m.し、その䞊柄液
を酵玠液ずする。 このようにしお埗られる酵玠液はマンナン加氎
分解酵玠、キシラン加氎分解酵玠およびポルフむ
ラン加氎分解酵玠を含有する。 本発明では䞊蚘培逊に圓り、海苔由来の倚糖類
ずしお䞻にマンナンもしくはキシランから成るも
のを誘導物質ずしお培地に含有させお䞻ずしおマ
ンナン加氎分解酵玠もしくはキシラン加氎分解酵
玠をそれぞれ培地䞭に生産させ、埗られる培逊液
からこれらの各酵玠を䞻ずしお含む酵玠液を調補
し、䞡者の酵玠液を組合せお海苔葉䜓のプロトプ
ラスト化に甚いるこずも可胜である。 なお、本発明で海苔葉䜓のプロトプラスト化に
マンナン加氎分解酵玠ずキシラン加氎分解酵玠を
䞻に甚いるのは、前者が海苔の衚局に存圚する顆
粒状のマンナンに䜜甚しお葉䜓に倧きく切断郚を
圢成しお现胞壁を圢成しおいるミクロフむブリル
圢態のキシランに察する埌者の䜜甚をし易くする
こずに基づくものであり、したが぀お、キシラン
加氎分解酵玠が海苔葉䜓のプロトプラスト化に最
も重芁な䜜甚をしおいるものず蚀える。なお、ポ
ルフむラン加氎分解酵玠は海苔葉䜓の现胞充間物
質ずしおのポルフむランに䜜甚しお分解するので
該酵玠を含む酵玠液を甚いるずプロトプラスト化
が䞀局促進される。 海苔葉䜓に䜜甚させる䞊蚘酵玠液の量は、海苔
葉䜓をcm皋床のもの〜枚に察し、䞊蚘酵玠
液を〜10倍に濃瞮したものの10ml皋床が適圓で
あり、〜時間の䜜甚で海苔のプロトプラスト
を調補し埗る。 たた、本発明では海苔葉䜓に䞊蚘酵玠液を䜜甚
させるに圓぀お、該葉䜓にプロテアヌれを䜜甚さ
せるず海苔の衚局を被芆しおいる蛋癜質の薄い局
を分解し埗るのでプロトプラストを調補するうえ
で䞀局効果的である。プロテアヌれずしおはパパ
むンが特に奜たしく、10のパパむン液ずしお葉
䜓に15〜30分皋床䜜甚させるず䞊蚘蛋癜質の薄局
を有効に分解、陀去し埗る。 なお、プロテアヌれの海苔葉䜓に察する䜜甚
は、䞊蚘プロトプラスト化のための酵玠液による
凊理に先立぀お行぀おもよく、又、該酵玠液によ
る凊理ず平行的に行぀おもよい。 䞊述のようにしお埗られる海苔のプロトプラス
トは海苔を物理的に切断するこずなく、酵玠凊理
によ぀おのみ調補されるものであるから健党な状
態であ぀お、现胞融合に利甚するのに適しおい
る。 䟋えば、本発明の方法で調補された海苔のプロ
トプラストをペトリ皿内で人工海氎藻類甚
Asp.12に懞濁させ、ペトリ皿の底郚に着生し
たプロトプラストの生育状況を芳察した結果によ
る生育状況に良奜である。 叙䞊のように、本発明によるず、海苔のプロト
プラストが酵玠的凊理のみで健党な状態で埗られ
るので、今埌の海苔の现胞融合技術の進展に益す
るものず蚀える。 以䞋に実斜䟋を瀺しお本発明を曎に具䜓的に説
明する。 実斜䟋  培地の調補 ペプトン 1.0重量 酵母゚キス 0.1  〃  K2HPO4 0.01 〃  FeCl3 0.6mg トリス緩衝液トリスアミノメタン
0.1重量 海苔の熱氎抜出残枣 1.0重量 䞊蚘組成のものを海氎に添加しおPH7.5に調敎
したものを培地に甚いた。 酵玠液の調補 䞊蚘培地にシナヌドモナスPseudomonas
sp埮工研条寄No.BP―330を接し、300r.p.m.の撹
拌䞋に通気しながら通気量2000mlmin25℃
で日間培逊を行぀た。 埗られた培逊液を℃の枩床で30分間遠心分離
10000r.p.m.し、その䞊柄液を10倍に濃瞮しお
酵玠液ずした。 このようにしお調補した酵玠液の難消化性倚糖
類に察する酵玠掻性を調べた結果は、䞋蚘衚に瀺
すずおりである。 なお、参考ずしお前述した藀田等の方法で甚い
た酵玠液の調補法を䞋蚘に瀺すずずもに、その酵
玠掻性を調べた結果も䜵せお衚瀺した。 酵玠液の調補法 培地組成 NH4NO3 0.1重量 K2HPO4 0.01 〃  FeCl3 0.6mg トリスアミノメタン 0.1重量 アサクサノリ粉末 0.2重量 䞊蚘組成を海氎に添加しおPHを7.5に調敎。 アサクサノリ粉末は別に滅菌しお添加した。 䞊蚘培地に、あらかじめ日間培逊した
Pseudomonas spの菌株を接皮し、25℃で日間
通気䞋に培逊を行ない、぀いで日間静眮培逊を
行぀たのち、埗られた培逊液をセラむトスタン
ダヌドスヌパヌセルで濟過、陀菌したものを酵
玠液ずした。 The present invention relates to a method for preparing healthy seaweed protoplasts, and more particularly, to a method for preparing seaweed protoplasts that can be effectively applied to cell fusion. In recent years, research into so-called cell fusion, the fusion between cells of different organisms, has become very active as a genetic engineering method, and some cases have already reached the stage of practical application in land plants. However, there are few research reports on cell fusion in seaweeds, especially in seaweeds, and no successful example has yet been found. Incidentally, although protoplasts of land plants such as wheat, barley, and soybeans can be easily prepared using commercially available enzymes (e.g., cellulase, macerozyme, etc.), enzymes that can convert linseed plants into protoplasts are not currently available. This is thought to be one of the reasons why cell fusion technology in laver species lags behind that of land plants. So far, as an attempt to convert laver to protoplasts, Fujita et al. reported on ``Isolation of protoplasts from laver and laver by enzyme treatment and their generation'' (Japan Fisheries Society, 1981). Autumn lecture abstracts, page 23,
213) can only be seen. In this method by Fujita et al., a crude enzyme solution obtained from a culture of Pseudomonas SP strain (strain P-1) is applied to leaf pieces obtained by physically shredding seaweed thallus for about 4 hours. However, in this method, the enzyme treatment to obtain protoplasts takes a long time, and the protoplasts obtained are unhealthy because the enzymes are applied to physically cut seaweed. Therefore, there is a possibility that cell fusion using these protoplasts will be hindered. However, in the cell fusion method, the health of the protoplasts used is a very important factor; if the protoplasts are unhealthy, the fusion rate during cell fusion will be low and the subsequent growth in culture will be affected. This is because it is thought that it will become inferior. In addition, the reason for cutting the seaweed thallus using the above method is that the enzyme produced by the Pseudomonas SP strain does not act on the surface layer of the seaweed, but acts from the cut part, breaking down the cell wall of the seaweed and forming protoplasts. It is thought that it is based on. According to a report by Preston et al., mannan exists in the form of granules on the surface of seaweed, the cell wall of seaweed is composed of xylan in the form of microfibrils, and porphyranes are thought to exist as a cell filling substance. Ru. Also, according to LAHanic et al., there is a thin coating of protein on the surface of seaweed. In other words, from the viewpoint of the structure of seaweed, it was thought that seaweed could not be transformed into protoplasts unless it was cut. The present inventor investigated the conversion of seaweed into protoplasts from the viewpoint that in order to obtain healthy seaweed protoplasts suitable for cell fusion, it is necessary to disintegrate the seaweed from its surface layer without physically cutting it. As a result, by treating seaweed with an enzyme solution containing at least mannan hydrolase and xylan hydrolase, or further containing polyphyllane hydrolase,
The present invention was made based on the knowledge that seaweed protoplasts can be prepared in a healthy state. That is, an object of the present invention is to provide a method for preparing healthy seaweed protoplasts that can be effectively applied to cell fusion. The present invention will be explained in detail below. The main structural features of the present invention are that seaweed fronds are
At least mannan hydrolase and xylan prepared from a culture solution obtained by culturing a microorganism capable of hydrolyzing indigestible polysaccharides belonging to the genus Pseudomonas in a medium containing seaweed or a seaweed-derived polysaccharide as an inducer. The process consists of treatment with an enzyme solution containing hydrolytic enzymes. Note that other configurations of the present invention will become clear from the following description. The microorganisms that have the ability to hydrolyze indigestible polysaccharides used in the preparation of the enzyme solution used in the protoplastization of seaweed in the present invention are those that are isolated from seawater and are used to It has the ability to hydrolyze porphyrane and has the following mycological properties. Mycological properties: Morphology Regarding cells grown in ZoBELL2216E medium, (a) The cell morphology is 0.5 to 1Ό in size for rods.
m x 1.5 to 2.5 ÎŒm (B) Motile, flagella are monopolar (C) Gram staining is negative Growth condition Growth condition in ZoBELL2216E slant medium, (B) Good at temperature of 20℃ to 27℃ (b) Deposit pale yellow pigment (c) Form filiform colonies Physiological properties (b) Catalase test positive (b) Oxidase test positive (c) Production of acid from glucose Positive ( d) O-F test (based on Hugh Leifson method)
0 (e) Vibro-Static Agent (0/129) Negative (f) Capacity to liquefy + (g) Xylan decomposition ability + (ch) Mannan decomposition ability + (li) Aerobicity In view of the above mycological properties, the present invention The microorganism utilized can be identified as a strain belonging to the genus Pseudomonas. This strain of Pseudomonas sp. PT-5 has been deposited with the National Institute of Microbiology, Agency of Industrial Science and Technology under accession number 330. In the present invention, the above-mentioned microorganism is cultured in a medium containing seaweed or seaweed-derived polysaccharide as an inducer to produce mannan hydrolase, xylan hydrolase, and porphyrane hydrolase in the medium. The term "polysaccharide derived from seaweed" as used herein refers to a residue mainly consisting of polysaccharides obtained by hot water extraction of seaweed to remove soluble components, or a residue obtained by further purification to increase the polysaccharide content. means something For example, seaweed is soaked in 10 times the amount of water, heated in an autoclave at 120°C for 30 minutes, then the soluble fraction is removed using a filter cloth, and the resulting residue is heated in the same manner as above to dissolve the soluble fraction. Repeat the operation of removing the segment (about 5 times), then immerse the resulting residue in 100% ethanol, leave it at room temperature overnight, remove the soluble segment, and dry it as a residue consisting of polysaccharides. Alternatively, the residue obtained by repeating the above heating and removal of the soluble fraction (not immersed in ethanol) is immersed in a 1N-NaOH solution, left overnight at room temperature, and then the soluble fraction is removed. The residue was diluted with NaOH
A polysaccharide obtained by extracting with a 20% hot aqueous solution, centrifuging the resulting extract, adding Fehling's solution to the supernatant to form a precipitate, and washing the precipitate with water to remove Cu ions. (mannan) or a polysaccharide (xylan) that is obtained by purifying the polysaccharide (xylan) that is obtained by adding HC1 to the supernatant liquid obtained by adding Fehling's solution to form a precipitate and adjusting the pH to 3. used as The appropriate amount of seaweed or seaweed-derived polysaccharide to be added to the medium as the inducer is 1 to 2% by weight. The medium used for culturing the above-mentioned microorganisms used in the present invention is prepared by dissolving the above-mentioned inducer as a carbon source, peptone and yeast extract as a nitrogen source, and K 2 HPO 4 , FeCl 3 and the like as inorganic substances in seawater or artificial seawater. , a buffer solution (for example, a Tris buffer with pH adjusted to around 7.5 is preferable. Examples of the culture medium composition are as follows.Medium composition: seaweed or seaweed-derived polysaccharide 1.0 (wt%) peptone 1.0 yeast extract 0.1 K 2 HPO 4 0.01 FeCl 3 0.6 mg/1 Tris buffer 0.1 (wt%) Dissolve in seawater at the above ratio and adjust the pH to 7.5. The culture conditions in the above medium for the above microorganisms used in the present invention are as follows: Aeration for 4 days at a temperature of 25℃, under stirring aeration (aeration rate 1000-2000ml/min, number of stirrings 100-
300r.pm). To prepare an enzyme solution from the culture solution obtained by culturing as described above, the culture solution is incubated at a temperature of 4°C.
Centrifuge for 30 minutes (10,000 rpm) and use the supernatant as the enzyme solution. The enzyme solution thus obtained contains mannan hydrolase, xylan hydrolase and porphyrane hydrolase. In the present invention, in the above culture, a polysaccharide derived from seaweed, mainly consisting of mannan or xylan, is contained in the medium as an inducer to mainly produce mannan hydrolase or xylan hydrolase, respectively, in the medium. It is also possible to prepare an enzyme solution mainly containing each of these enzymes from the culture solution obtained, and to use the combination of both enzyme solutions for protoplast formation of seaweed thallus. In addition, in the present invention, mannan hydrolase and xylan hydrolase are mainly used to convert the seaweed thallus into protoplasts. This is based on facilitating the latter action on the microfibrillar form of xylan that forms the cell wall. It can be said that it is working. In addition, since porphyrane hydrolase acts on and decomposes porphyrane as a cell-filling substance of the seaweed thallus, protoplast formation is further promoted when an enzyme solution containing this enzyme is used. The appropriate amount of the enzyme solution to act on the seaweed leaves is about 10 ml of the enzyme solution concentrated 5 to 10 times for 4 to 5 pieces of seaweed leaves of about 5 cm. Seaweed protoplasts can be prepared as a function of time. In addition, in the present invention, when the above-mentioned enzyme solution is applied to the seaweed thallus, it is possible to degrade the thin layer of protein covering the surface layer of the seaweed by allowing the protease to act on the thallus, which is useful for preparing protoplasts. It is even more effective. As the protease, papain is particularly preferred, and the thin layer of the above protein can be effectively decomposed and removed by acting on the thallus as a 10% papain solution for about 15 to 30 minutes. The action of protease on the seaweed fronds may be carried out prior to the above-mentioned treatment with the enzyme solution for protoplast formation, or may be carried out in parallel with the treatment with the enzyme solution. The seaweed protoplasts obtained as described above are prepared only by enzymatic treatment without physically cutting the seaweed, so they are in a healthy state and suitable for use in cell fusion. There is. For example, seaweed protoplasts prepared by the method of the present invention are placed in artificial seawater (for algae) in a Petri dish.
The growth status of protoplasts suspended in Asp.12) and attached to the bottom of a Petri dish was observed, and the growth status was found to be good. As mentioned above, according to the present invention, seaweed protoplasts can be obtained in a healthy state only by enzymatic treatment, and therefore it can be said to be beneficial for the future advancement of seaweed cell fusion technology. EXAMPLES The present invention will be explained in more detail with reference to Examples below. Example 1 Preparation of medium Peptone 1.0 (wt%) Yeast extract 0.1 (〃) K 2 HPO 4 0.01 (〃) FeCl 3 0.6 mg/1 Tris buffer (tris aminomethane)
0.1 (wt%) Hot water extraction residue of seaweed 1.0 (wt%) The above composition was added to seawater and adjusted to pH 7.5 and used as a culture medium. Preparation of enzyme solution Add Pseudomonas to the above medium.
25℃ while aerating with 300rpm stirring (air flow rate 2000ml/min)
Culture was carried out for 4 days. The obtained culture solution was centrifuged (10,000 rpm) at a temperature of 4° C. for 30 minutes, and the supernatant was concentrated 10 times to obtain an enzyme solution. The results of examining the enzyme activity of the enzyme solution thus prepared against indigestible polysaccharides are shown in the table below. For reference, the preparation method of the enzyme solution used in the method of Fujita et al. mentioned above is shown below, and the results of investigating the enzyme activity are also displayed. Preparation method of enzyme solution: Medium composition NH 4 NO 3 0.1 (wt%) K 2 HPO 4 0.01 (〃 ) FeCl 3 0.6 mg/1 Tris-aminomethane 0.1 (wt%) Asakusanori powder 0.2 (wt%) The above composition was mixed with seawater and adjust the pH to 7.5. Asakusanori powder was sterilized and added separately. Cultured in the above medium for 2 days in advance.
A strain of Pseudomonas sp was inoculated and cultured at 25°C for 5 days under aeration, followed by static culture for 2 days, and the resulting culture solution was filtered through Celite (Standard Super Cell) to remove bacteria. was used as the enzyme solution.

【衚】 衚にみられるように、本発明で甚いる酵玠液は
マンナンおよびキシランに察する掻性が藀田等の
方法で甚いた酵玠液に比し優れおいる。 プロトプラストの調補 海苔葉䜓をcm皋床のもの〜枚を型詊隓
管に入れ、これに䞊蚘酵玠液10mlを加えお海苔葉
䜓を該酵玠液に浞挬しながら、20℃の枩床でモノ
ヌ型振盪噚を甚いお時間振盪70ストロヌク
分させお海苔のプロトプラストを埗た。 実斜䟋  本䟋は海苔葉䜓のプロトプラスト化に圓぀お該
葉䜓にパパむンを䜜甚させた䟋を瀺したものであ
る。なお、パパむンを葉䜓に䜜甚させるほかは、
実斜䟋ず同様な手順でプロトプラストの調補を
行぀た。 パパむンによる凊理 型詊隓管にcm皋床の海苔葉䜓の〜枚を
収容し、これに10パパむン溶液酢酞塩バツフ
アヌに溶解しおPH6.0にしたもの10mlを添加し
お海苔葉䜓を該パパむン溶液に浞挬しながら、25
℃の枩床で20分間振盪モノヌ型振盪噚70ストロ
ヌク分させた。 プロトプラストの調補 䞊述のようにしおパパむンを䜜甚させた海苔葉
䜓を、実斜䟋に蚘茉した手順に埓぀お酵玠液で
60分間凊理しおプロトプラストを調補した。[Table] As seen in the table, the enzyme solution used in the present invention has superior activity against mannan and xylan compared to the enzyme solution used in the method of Fujita et al. Preparation of protoplasts: Place 4 to 5 pieces of seaweed fronds of approximately 5cm in an L-shaped test tube, add 10ml of the above enzyme solution to this, and while immersing the nori fronds in the enzyme solution, incubate at a temperature of 20°C. Shake for 4 hours using a type shaker (70 strokes/
minutes) to obtain seaweed protoplasts. Example 2 This example shows an example in which papain was applied to seaweed thallus during protoplast formation. In addition, in addition to making papain act on the thallus,
Protoplasts were prepared in the same manner as in Example 1. Treatment with papain Place 4 to 5 sheets of nori fronds approximately 5 cm in length in an L-shaped test tube, add 10 ml of 10% papain solution (dissolved in acetate buffer to pH 6.0), While immersing the leaf in the papain solution,
It was shaken for 20 minutes (70 strokes/min on a monoshaft shaker) at a temperature of .degree. Preparation of protoplasts The seaweed thallus treated with papain as described above was treated with an enzyme solution according to the procedure described in Example 1.
Protoplasts were prepared by treating for 60 minutes.

Claims (1)

【特蚱請求の範囲】  海苔葉䜓を、シナヌドモナス属
Pseudomonasに属する難消化性倚糖類の加氎
分解胜を有する埮生物を、海苔もしくは海苔由来
の倚糖類を誘導物質ずしお含む培地䞭で培逊しお
埗られる培逊液から調補した少なくずもマンナン
加氎分解酵玠ずキシラン加氎分解酵玠ずを含有す
る酵玠液で凊理するこずを特城ずする海苔のプロ
トプラストを調補する方法。  前蚘酵玠液による凊理に先立ち、海苔葉䜓を
プロテアヌれで凊理する特蚱請求の範囲第項蚘
茉の方法。  前蚘酵玠液による凊理ず平行しお、海苔葉䜓
をプロテアヌれで凊理する特蚱請求の範囲第項
蚘茉の方法。  海苔由来の倚糖類が海苔を熱氎抜出しお埗ら
れる倚糖類含有残枣である特蚱請求の範囲第項
乃至第項のいずれか項に蚘茉の方法。  海苔由来の倚糖類が海苔を熱氎抜出しお埗ら
れる残枣を粟補凊理したものである特蚱請求の範
囲第項乃至第項のいずれか項に蚘茉の方
法。  前蚘酵玠液がポルフむラン加氎分解酵玠も含
有するものである特蚱請求の範囲第項乃至第
項のいずれか項に蚘茉の方法。  前蚘酵玠液がマンナン加氎分解酵玠を含有す
る酵玠液ずキシラン加氎分解酵玠を含有する酵玠
液ずを組合せたものである特蚱請求の範囲第項
乃至第項のいずれか項に蚘茉の方法。  培地が窒玠源ずしおペプトンおよび酵母゚キ
スを含有するものである特蚱請求の範囲第項乃
至第項のいずれか項に蚘茉の方法。  プロテアヌれがパパむンである特蚱請求の範
囲第項又は第項蚘茉の方法。[Scope of Claims] 1 A seaweed thallus is cultured in a medium containing seaweed or seaweed-derived polysaccharide as an inducer using a microorganism having the ability to hydrolyze indigestible polysaccharides belonging to the genus Pseudomonas. A method for preparing seaweed protoplasts, which comprises treating with an enzyme solution containing at least mannan hydrolase and xylan hydrolase prepared from the obtained culture solution. 2. The method according to claim 1, wherein the seaweed thallus is treated with protease prior to the treatment with the enzyme solution. 3. The method according to claim 1, wherein the seaweed thallus is treated with protease in parallel with the treatment with the enzyme solution. 4. The method according to any one of claims 1 to 3, wherein the polysaccharide derived from seaweed is a polysaccharide-containing residue obtained by hot water extraction of seaweed. 5. The method according to any one of claims 1 to 3, wherein the polysaccharide derived from seaweed is obtained by purifying a residue obtained by hot water extraction of seaweed. 6 Claims 1 to 3, wherein the enzyme solution also contains porphyrane hydrolase.
The method described in any one of paragraphs. 7. The enzyme solution according to any one of claims 1 to 3, wherein the enzyme solution is a combination of an enzyme solution containing a mannan hydrolase and an enzyme solution containing a xylan hydrolase. Method. 8. The method according to any one of claims 1 to 3, wherein the medium contains peptone and yeast extract as nitrogen sources. 9. The method according to claim 2 or 3, wherein the protease is papain.
JP58149378A 1983-08-16 1983-08-16 Preparation of laver protoplast Granted JPS6041485A (en)

Priority Applications (1)

Application Number Priority Date Filing Date Title
JP58149378A JPS6041485A (en) 1983-08-16 1983-08-16 Preparation of laver protoplast

Applications Claiming Priority (1)

Application Number Priority Date Filing Date Title
JP58149378A JPS6041485A (en) 1983-08-16 1983-08-16 Preparation of laver protoplast

Publications (2)

Publication Number Publication Date
JPS6041485A JPS6041485A (en) 1985-03-05
JPS6257306B2 true JPS6257306B2 (en) 1987-11-30

Family

ID=15473820

Family Applications (1)

Application Number Title Priority Date Filing Date
JP58149378A Granted JPS6041485A (en) 1983-08-16 1983-08-16 Preparation of laver protoplast

Country Status (1)

Country Link
JP (1) JPS6041485A (en)

Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPH02117607U (en) * 1989-03-07 1990-09-20

Families Citing this family (2)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPH0654071B2 (en) * 1989-11-25 1994-07-20 立山アルミニりム工業株匏䌚瀟 Combination bay window device
JP2008125422A (en) * 2006-11-20 2008-06-05 Mie Prefecture Method for converting dried laver seaweed into single cell form, and culturing the same

Citations (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPS5421427A (en) * 1977-07-18 1979-02-17 Mitsubishi Electric Corp Unsaturated polyester varinish composition with low odor

Patent Citations (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPS5421427A (en) * 1977-07-18 1979-02-17 Mitsubishi Electric Corp Unsaturated polyester varinish composition with low odor

Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
JPH02117607U (en) * 1989-03-07 1990-09-20

Also Published As

Publication number Publication date
JPS6041485A (en) 1985-03-05

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